BRUNO MARTINS DALA PAULA
Efeitos do Huanglongbing (HLB) na composição
química e características sensoriais de suco de
laranja
Faculdade de Farmácia da UFMG
Belo Horizonte, MG
2017
BRUNO MARTINS DALA PAULA
Efeitos do Huanglongbing (HLB) na composição
química e características sensoriais de suco de
laranja
Tese apresentada ao Programa de Pós-Graduação em
Ciência de Alimentos da Faculdade de Farmácia da
Universidade Federal de Minas Gerais, como requisito parcial
à obtenção do grau de doutor.
Orientadora: Profª. Drª. Maria Beatriz Abreu Glória
Tutores no exterior: Dra. Anne Plotto e Dr. John A. Manthey
Faculdade de Farmácia da UFMG
Belo Horizonte, MG
2017
Dala Paula, Bruno Martins.
D136e
Efeitos do Huanglongbing (HLB) na composição química e
características sensoriais de suco de laranja / Bruno Martins
Dala Paula. – 2017.
131 f. : il.
Orientadora: Maria Beatriz Abreu Glória. Tutores: Anne Plotto, John A. Manthey.
Tese (doutorado) - Universidade Federal de Minas Gerais, Faculdade de Farmácia, Programa de Pós-Graduação em Ciência de Alimentos.
1. Suco de laranja – Indústria – Teses. 2. Alimentos – Análise – Teses. 3. Alimentos – Avaliação sensorial – Teses. 4. Alimentos – Composição – Teses. 5. Alimentos –Qualidade – Teses. 6. Frutas cítricas – Doenças e pragas –Teses. 7. Huanglongbing (HLB) – Doença – Teses. I. Glória, Maria Beatriz Abreu. II. Plotto, Anne. III. Manthey, John A. IV. Universidade Federal de Minas Gerais. Faculdade de Farmácia. V. Título.
CDD: 664
À minha família, orientadora, tutores, e
aos que estiveram ao meu lado dedico
com muito entusiasmo e gratidão este
trabalho.
AGRADECIMENTOS
Aos meus pais (Gilberto e Edite) pelo amor e suporte constante, além dos
ensinamentos que foram a base para a formação de quem hoje eu sou. Às minhas irmãs (Roberta e Karina) e sobrinhos (Fernando e Guilherme) por compartilharem seus valiosos momentos e tornar meus dias mais prazerosos. À professora Maria Beatriz Abreu Glória, por acreditar em meu trabalho e assim contribuir para a reconstrução da minha autoestima, pelo altruísmo em compartilhar os seus conhecimentos e saberes. Por se um exemplo de profissional a ser seguido. Aos meus tutores no exterior Dra. Anne Plotto e Dr. John Manthey pela amizade e companheirismo dentro e fora dos laboratórios. Foram muitos os aprendizados e momentos de reflexões, muito obrigado! Ao Lucian Ferry, agradeço pelo companheirismo e por toda ajuda oferecida, principalmente com as inúmeras revisões da escrita no idioma inglês. Aos amigos de todas as horas que sempre me apoiaram e compreenderam as minhas ausências, muitas vezes motivadas por compromissos acadêmicos. Obrigado a: Abel, Alessandra Santos, Ana Lígia, Clayson Pereira, Christiano Moreira, Cristiano Araújo, Danielle Vasconcelos, Débora Figueiredo, Dhionne Gomes, Diogo Satiro, Emmanuel Almada, Fernanda Louro, Gustavo Medeiros, Hélio Navarro, Kênia Roberta, Luana Oliveira, Luiz Machado, Marco Polo, Nathália Botelho, Pollyana Castro, Sheyla França, Thiago Andrade, Tiago Sial, Valcir. Aos amigos e companheiros dessa aventura que é o mundo acadêmico, que conhecem bem as dificuldades e que nunca deixaram de me motivar com palavras de conforto e um sorriso no rosto: Adriana Correa, Aisa Del Rio, Andrezza Estevam, Arthur Magno, Cyntia Barreto, Caroline Paiva, Cecília Bandeira, Edneia Xavier, Fabiana Diniz, Flávia Custódio, Gisela Machado, Guilherme Reis, José Maria, Juliana Rigueira, Larissa Bomtempo, Laura Ciribelli, Patrícia Tette, Paula Santiago, Raquel Braga, Regina Adão, Regina Carvalho, Ricardo Byrro, Rummenigge Oliveira, Silvia Vieira, Tânia Silveira, Tarliane Silva e Warlley Evangelista. Aos professores que compartilharam os seus conhecimentos. Todos que contribuíram com o meu crescimento pessoal, acadêmico e profissional. Aos pesquisadores, técnicos e amigos do USDA, Fort Pierce pelo auxílio na pesquisa e suporte durante a minha estadia no USDA: Dr. Liz Baldwin, Dr. Jinhe Bai, Dr. Hong Chen, Carly Franko, Marcus Reis, Veronica Cook, Dave e Kimberly Wood, Dr. Chris Ference, Nancy Owen, Holly Sisson, Elena Branca, XiuXiu Sun. À minha mãe Americana, Jackie White e Bob pelo caloroso acolhimento e por serem exemplos de pessoas gentis e generosas. Aos amigos Sai Xu, Valentina Candia, Sajid Ali, Hernandes Burgos, Sheree Deal e Mathew por fazerem parte de um momento muito especial da minha vida. Aos funcionários da Faculdade de Farmácia por todo o auxílio prestado. Ao Conselho Nacional de Desenvolvimento Científico e Tecnológico (CNPq).
Muito obrigado!
“One looks back with appreciation to the
brilliant teachers, but with gratitude to
those who touched our human feelings.
The curriculum is so much necessary
raw material, but warmth is the vital
element for the growing plant and for the
soul of the child” (Carl Jung)
6
SUMÁRIO
SUMÁRIO ............................................................................................... 6
LISTA DE TABELAS ............................................................................. 9
LISTA DE FIGURAS ............................................................................ 11
LISTA DE ABREVIATURAS E SIGLAS ............................................. 13
RESUMO .............................................................................................. 14
ABSTRACT .......................................................................................... 15
INTRODUÇÃO GERAL ....................................................................... 16
REVISÃO DA LITERATURA ............................................................... 18
1. CLASSIFICAÇÃO TAXONÔMICA DA LARANJA E PRINCIPAIS CULTIVARES
PLANTADAS NO BRASIL ................................................................................... 18
2. BREVE HISTÓRICO DO CULTIVO E PRODUÇÃO DE LARANJA ................. 20
3. OCORRÊNCIA E EFEITO DA HUANGLONGBING NOS POMARES DE
LARANJA ............................................................................................................ 23
4. BREVE HISTÓRICO DA PRODUÇÃO DE SUCO DE LARANJAS .................. 26
5. ETAPAS DO PROCESSAMENTO E COMERCIALIZAÇÃO DO SUCO DE
LARANJA PRODUZIDO NO BRASIL .................................................................. 29
6. CONSUMO DA LARANJA IN NATURA E SEUS DERIVADOS ....................... 35
7. COMPOSIÇÃO QUÍMICA E NUTRICIONAL DO SUCO DE LARANJA ........... 37
8. PROPRIEDADES FUNCIONAIS DA LARANJA .............................................. 41
OBJETIVOS ......................................................................................... 43
CAPÍTULO I - INFLUENCE OF HARVEST TIME ON QUALITY OF
‘VALENCIA’ ORANGES AND JUICE, SECOND SEASON .............. 44
ABSTRACT ......................................................................................................... 44
1. INTRODUCTION............................................................................................. 45
2. MATERIAL AND METHODS ........................................................................... 46
2.1 Fruit sampling .......................................................................................... 46
2.2 Peel color and juice content analysis ........................................................ 46
2.3 Sugar and acid analysis ........................................................................... 46
2.4 Secondary metabolite analysis ................................................................. 47
2.5 Peel oil, pectin and pectinmethylesterase (PME)...................................... 47
2.6 Volatile analysis ....................................................................................... 47
2.7 Bioactive amines ...................................................................................... 48
2.8 Statistical analysis .................................................................................... 48
7
3. RESULTS AND DISCUSSION ........................................................................ 48
3.1 Peel color and juice content ..................................................................... 48
3.2 Peel oil and PME activity and pectin......................................................... 49
3.3 Sugars and acids ..................................................................................... 50
3.4 Secondary metabolites ............................................................................. 51
3.5 Bioactive amines ...................................................................................... 53
3.6 Volatiles ................................................................................................... 54
4. CONCLUSION ................................................................................................ 58
CAPÍTULO II - EFFECT OF HUANGLONGBING (GREENING
DISEASE) ON ORANGE JUICE QUALITY, A REVIEW .................... 59
ABSTRACT ......................................................................................................... 59
KEYWORDS ....................................................................................................... 59
1. INTRODCUTION............................................................................................. 60
2. WORLDWIDE CONSUMPTION AND PRODUCTION OF FRESH ORANGES
AND ORANGE JUICE ......................................................................................... 60
3. A BRIEF HISTORICAL BACKGROUND OF HUANGLONGBING INCIDENTS 61
5. SYMPTOMS OF HUANGLONGBING AND ITS IMPACT ON ORANGE TREES
........................................................................................................................... 68
6. FRESH ORANGES AND ORANGE JUICE QUALITY AFFECTED BY
CANDIDATUS LIBERIBACTER ASIATICUS ..................................................... 72
6.1 Effects on physicochemical and biochemical characteristics .................... 72
6.1.1 Peel color .......................................................................................... 72
6.1.2 Physicochemical characteristics ........................................................ 73
6.1.3 Sugars and organic acids .................................................................. 75
6.1.4 Secondary metabolites...................................................................... 76
6.1.5 Amino acids and bioactive amines .................................................... 80
6.2 Effects on sensory characteristics ............................................................ 81
6.3 Effect on the levels and profile of volatile compounds .............................. 86
6.4 Huanglongbing control and mitigation of its symptoms ............................. 87
7. FINAL CONSIDERATIONS ............................................................................ 88
CAPÍTULO III - ACTIVE TASTE COMPOUNDS IN JUICE MADE
FROM ORANGES SYMPTOMATIC OF HUANGLONGBING (HLB)
GREENING DISEASE ......................................................................... 90
ABSTRACT ......................................................................................................... 90
1. INTRODUCTION............................................................................................. 91
2. MATERIAL AND METHODS ........................................................................... 93
2.1 Juice samples .......................................................................................... 93
2.1.1 Sample preparation .......................................................................... 93
8
2.1.2 DNA extraction and qPCR detection of CLas from juice ................... 93
2.2 Chemical analysis of COJ and HLBOJ ..................................................... 93
2.2.1 Titratable acidity and soluble solids .................................................. 93
2.2.2 Total sugar, sucrose, glucose and fructose ...................................... 94
2.2.3 Citric acid, malic acid and ascorbic acid analyses ............................ 94
2.2.4 Secondary metabolites analyses ...................................................... 95
2.3 Fractionation of phenolic compounds from orange juice ........................... 95
2.3.1 Preparation of phenolic compound extracts of COJ and HLBOJ ...... 95
2.3.2 Fractionation of phenolic compound extracts by Fast Centrifugal
Partition Chromatography (FCPC) ............................................................ 96
2.3.3 Chemical characterization of phenolic compounds by HPLC– MS ... 96
2.3.4 Sub-fractionation of fractions A and B by HPLC ............................... 97
2.4 Sensory evaluation ................................................................................... 98
2.4.1 Comparative sensory analysis of COJ and HLBOJ .......................... 98
2.4.2 Descriptions of flavor attributes of fractions obtained from COJ and
HLBOJ ...................................................................................................... 98
2.5 Statistical analyses ................................................................................. 100
3. RESULTS ..................................................................................................... 100
4. DISCUSSION ................................................................................................ 108
5. CONCLUSION .............................................................................................. 110
CONCLUSÕES INTEGRADAS ......................................................... 111
REFERÊNCIAS BIBLIOGRÁFICAS ................................................. 112
PRODUÇÃO CIENTÍFICA DURANTE O DOUTORADO ................. 131
9
LISTA DE TABELAS
REVISÃO DA LITERATURA
Tabela 1. Características das principais cultivares de laranjas plantadas no Brasil
........................................................................................................................... 19
Tabela 2. Área destinada à colheita de laranja em hectares e quantidade
produzida em mil toneladas no Brasil, durante os anos de 2010 a 2017*........... 21
Tabela 3. Composição química representativa da laranja Valência in natura e do
seu suco. ........................................................................................................... 38
Tabela 4. Teores médios de flavonoides em casca, em vesícula de suco e em
laranja Valência ................................................................................................. 39
CAPÍTULO I
Table 1. Effect of harvest time on volatile abundance in ‘Valencia’ orange juice
(2012)z ............................................................................................................... 55
CAPÍTULO II
Table 1. Worldwide distribution of Huanglongbing’s bacteria and vectors. ......... 63
Table 2. Effects on diameter, weight and juice content in fruit affected by
Huanglongbing. .................................................................................................. 71
Table 3. Physicochemical characteristics of Valencia orange juice made with
healthy fruit and fruit at different stages of HLB infection. ................................... 74
Table 4. Physicochemical characteristics of Hamlin orange juice made with
healthy fruit and fruit at different stages of HLB infection. ................................... 75
Table 5. Sugars and acids of Valencia orange juice made with healthy fruit and
fruit at different stages of HLB infection. ............................................................. 77
10
CAPÍTULO III
Table 1. Mobile phases gradients (1 and 2) used to separate fractions A and B:
from healthy and huanglongbing (HLB)-affected Valencia orange juice into sub
fractions. ............................................................................................................ 97
Table 2. Descriptors and reference standards with suggested intensity for orange
juice sensory descriptive panel, using a 16-point intensity scale* ....................... 99
Table 3. Sensory descriptors of each sub-fraction (SF) obtained from A-COJ and
A-HLBOJ from healthy and huanglongbing (HLB)-affected Valencia orange juice,
respectively. ..................................................................................................... 105
Table 4. Sensory descriptors and concentration of each sub-fraction obtained
from B-COJ and B-HLBOJ from healthy and huanglongbing (HLB)-affected
Valencia orange juice, respectively .................................................................. 107
11
LISTA DE FIGURAS
REVISÃO DE LITERATURA
Figura 1. Esquema de uma planta de processamento comercial de suco de
laranja.. .............................................................................................................. 31
Figura 2. Exportações de FCOJ equivalente em toneladas por ano civil a partir
do porto de Santos.. ........................................................................................... 34
Figura 3. Exportações de NFC equivalente em toneladas por ano civil a partir do
porto de Santos.. ................................................................................................ 35
CAPÍTULO I
Figure 1. Changes of peel color (a*/b* ratio) and juice content of ‘Valencia’
orange fruit harvest from February to May 2012. ................................................ 49
Figure 2. Changes of peel oil content, pectin methylesterase (PME) activity, and
total pectin (galacturonic acid) content in ‘Valencia’ orange juice extracted from
fruit harvested from February to May 2012. ........................................................ 49
Figure 3. Changes of soluble solids content (SSC), titrable acidity (TA), and
SSC/TA ratio in ‘Valencia’ orange juice extracted from fruit harvested from
February to May 2012. ....................................................................................... 50
Figure 4. Changes of citric, malic, and ascorbic acids in ‘Valencia’ orange juice
extracted from fruit harvested from February to May 2012. ................................ 51
Figure 5. Changes of flavonoid glycosides (FGs, relative peak área) in ‘Valencia’
Orange juice extracted from fruit harvested from February to May 2012.
Hesperedin-4’-glucoside; hesperidin; 6,8-di-C-glucosyl apigenin; isosakuranetin
rutinoside; narirutin............................................................................................. 52
Figure 6. Changes of polymethoxylated flavones (PMFs, relative peak área) in
‘Valencia’ Orange juice extracted from fruit harvested from February to May
2012. Heptamethoxyflavone; quercetagetin hexamethylether; nobiletin;
tetramethylscutellarein; sinesetin; and tangeretin. .............................................. 52
Figure 7. Changes of limonoids (relative peak área) in ‘Valencia’ orange juice
extracted from fruit harvested from February to May 2012. Obacunone glucoside;
12
nomilin glucoside; nomilinic acid glucoside; limonin glucoside; limonin; and
nomilin. .............................................................................................................. 53
Figure 8. Changes of putrescine, spermidine, and spermine in ‘Valencia’ orange
juice extracted from fruit harvested from February to May 2012. ........................ 53
CAPÍTULO II
Figure 1. Countries currently affected by Huanglongbing – HLB.. ...................... 62
Figure 2. Development stages of Diaphorina citri Kuwayama (Hemiptera:
Psyllidae) and Trioza etrytreae (Del Guercio) (Hemiptera: Triozidae) .. .............. 67
Figure 3. HLB symptomatic orange leaves: symptomatic normal sized leaves with
development of blotchy-mottle; and symptomatic small sized leaves. ................ 69
Figure 4. Typical HLB symptomatic orange: asymmetric fruit containing small,
brownish aborted seeds; normal change of color in a healthy orange, CLas (-);
and inversion of colors in a typical HLB symptomatic orange, CLas (+). ............ 70
Figure 5. Symptomatic and asymptomatic orange of HLB disease, CLas (+); and
healthy oranges, CLas (-). .................................................................................. 72
CAPÍTULO III
Figure 1 Sensory scores (average ± standard deviation for 12 trained panelists)
for Valencia orange juice from healthy (COJ) or HLB-affected (HLBOJ) fruit.. .. 101
Figure 2. Quality attributes (average ± standard deviation for four replicates) in
Valencia orange juice from healthy (COJ) or HLB-affected (HLBOJ) fruit.. ....... 102
Figure 3. Secondary metabolites (average ± standard deviation for three
replicates) in Valencia orange juice from healthy (COJ) or HLB-affected (HLBOJ)
fruit.. ................................................................................................................. 103
Figure 4. HPLC chromatograms of healthy (COJ) (a) or huanglongbing (HLB)-
affected (HLBOJ) (b) Valencia orange juice from fraction A showing 10 sub-
fractions with their respective lowest concentration at which taste was perceived.
......................................................................................................................... 104
13
LISTA DE ABREVIATURAS E SIGLAS
A-COJ Fraction A of COJ
A-HLBOJ Fraction A of HLBOJ
APTA Agência Paulista de Tecnologia dos Agronegócios
AT Acidez titulável
B-COJ Fraction B of COJ
B-HLBOJ Fraction B of HLBOJ
CDA Coordenadoria de Defesa Agropecuária
CL Candidatus Liberibacter
CLaf Candidatus Liberibacter africanus
CLam Candidatus Liberibacter americanus
CLas Candidatus Liberibacter asiaticus
COJ Control juice
CVC Clorose variegada dos citros
FCOJ Frozen concentrated orange juice
FCPC Fast centrifugal partition chromatography
FG Flavonoid glycosides
Fundecitrus Fundo de Defesa da Citrucultura
GC-MS Gas chromatography-mass spectrometry
HCA Hydroxycinnamic acids
HLB Huanglongbing
HLBOJ HLB orange juice
HPLC High performance liquid chromatography
IBGE Instituto Brasileiro de Geografia e Estatística
MAPA Ministério da Agricultura, Pecuária e Abastecimento
MG Minas Gerais
MS Mass-spectrometry
NFC Not from concentrate juice
PCR Polymerase chain reaction
PDA Photodiode array
PME Pectinmethylesterase
PMF Polymethoxylated flavones
SIDRA Sistema IBGE de Recuperação Automática
SP São Paulo
SPME Solid phase microextraction
SSC Soluble solids content
SS Sólidos solúveis
TA Titratable acidity
14
RESUMO
Huanglongbing (HLB) é a mais severa doença em citros no mundo. Sintomas dessa
doença incluem ramos com folhas amareladas, queda precoce e alteração das
características sensoriais dos frutos, desfolhamento e morte prematura da árvore. Este
trabalho teve como objetivos determinar as alterações físico-químicas, na composição
química e nas características sensoriais no suco de laranja acometido pelo HLB, assim
como investigar as causas do amargor no suco de laranja, além daquelas provenientes
da limonina e nomilina. Foi realizado um estudo avaliativo das características físico-
químicas e bioquímicas de sucos de laranjas Valência colhidas em diferentes meses
(fevereiro, março, abril e maio) numa mesma safra (2012). Confirmaram-se as
alterações nos parâmetros estudados, sendo as colhidas no meio da estação mais
adequadas ao processamento. Em seguida foi realizada uma revisão de literatura sobre
os efeitos do HLB nos parâmetros físico-químicas, composição química e
características sensoriais de suco de laranja, assim como a determinação laboratorial
das mesmas. Tanto a revisão quanto as análises químicas demonstraram aumento da
acidez titulável (AT), conteúdos de ácido cítrico, limonina e nomilina, dentre outros
metabólitos secundários e redução dos sólidos solúveis (SS), ratio, açúcares e teores
de ácido málico. Os sucos provenientes de laranjas sintomáticas para o HLB
apresentaram maior intensidade dos seguintes atributos sensoriais: sabores amargo,
ácido, metálico e umami; aromas de toranja, de casca de laranja e de suco envelhecido;
e das sensações bucais de adstringência, queimação e formigamento. Foi realizado um
fracionamento dos compostos não-voláteis do suco de laranja, com subsequente
descrição sensorial dos mesmos. Verificou-se sabor amargo em uma fração onde a
limonina e nomilina estavam presentes, mas também em outras com predomínio de
ácidos hidroxicinâmicos e ausência dos limonoides. Essa é uma evidência de que
outro(s) composto(s), possivelmente algum ácido hidroxicinâmico, esteja(m)
envolvido(s) com o típico amargor conferido pelo HLB.
PALAVRAS-CHAVE: Huanglongbing. Suco de laranja. Amargor. Qualidade de
alimentos. Análise sensorial
15
ABSTRACT
Huanglongbing (HLB) is the most severe citrus disease in the world. Symptoms
of HLB include branches with yellow leaves, premature dropping and changes in
fruit sensory quality, loss of leaves and premature death of the tree. The
objectives of this work were to evaluate the physicochemical, chemical
composition and sensory changes in juice made with HLB symptomatic oranges,
as well as to investigate the causes of the bitterness found in HLB orange juice,
other than the bitter limonoids, limonin and nomilin. The physicochemical
caracteristics and chemical composition were evaluated in juice made with
Valencia oranges harvested throughout the season (February, March, April and
May 2012). This study confirmed the changes of some chemical composition
over the harvest season, with better attributes for processing in the mid-season.
Then, a literature review and laboratory analysis evaluating the effects of HLB on
physicochemical, chemical composition and sensory characteristics were
conducted. Both, review and laboratory analysis, revealed increases of titratable
acid (TA), levels of citric acid, limonin and nomilin, among other secondary
metabolites, and a decrease of soluble solid contents (SSC), SSC/TA, sugars
and malic acid contents. The juice from HLB symptomatic oranges had higher
values for the sensory attributes: bitterness, sourness, metallic and umami
tastes; flavors of grapefruit, orange peel and staleness; and astringent, burning
and tingling month-feels compared to healthy juice. Non-volatile compounds
were extracted from Valencia orange juice and fractionated and sensorially
described. Bitterness was detected in the fraction containing limonin and nomilin
as well as in fractions which did not contain these limonoids, but prevalence of
hydroxycinnamic acids. This evidences the existence of other compounds,
possibly hydroxycinnamate acids, involved with the typical HLB-bitterness.
KEYWORDS: Huanglongbing. Orange juice. Bitterness. Food quality. Sensory
evaluation.
16
INTRODUÇÃO GERAL
O suco de laranja é a bebida mais consumida no mundo dentre os sucos
de frutas, com participação de 45% no mercado (MARKESTRAT, 2016). O Brasil
é o maior produtor mundial de laranjas e possui destaque no mercado
internacional da fruta in natura, assim como de seu suco. No entanto, no período
de 2011 a 2017, o país apresentou redução de aproximadamente 13,2% na
safra de laranjas, e tendência de queda na área destinada ao cultivo da fruta,
apesar do incentivo da demanda internacional pela laranja brasileira nos anos de
2016 e 2017, em decorrência do acentuado declínio da produção norte-
americana da fruta, em especial no estado da Flórida (IBGE/SIDRA, 2017;
USDA/FAS, 2017).
No entanto, atualmente os produtores citrícolas brasileiros e norte-
americanos estão enfrentando sérios problemas com a incidência da doença
Huanglongbing (HLB), também conhecida como “greening” dos citros em suas
plantações. Esta doença teve o seu primeiro relato na China no fim do século
XIX, no entanto, em 1966 foi realizado um estudo retrospectivo da situação dos
citros na Índia, sendo o HLB apontado como uma das principais causas do
gradual declínio das árvores cítricas ocorrido durante o século XVIII (FRASER et
al., 1966). A doença foi notificada na África do Sul no início do século XX,
estando atualmente presente em diversos países. Até 2004 não havia relatos
nas áreas mediterrâneas da Europa e nas Américas, quando a doença foi
detectada em vários pomares de São Paulo, sendo também notificada no ano
seguinte nos Estados Unidos - EUA (RAITHORE et al., 2015; TEIXEIRA et al.,
2005a; BOVÉ, 2006).
O HLB é mundialmente considerado a doença mais grave que acomete
os citros e, consequentemente, um sério problema para a indústria de
processamento dos mesmos. A doença está associada com a presença da
bactéria gram negativa do gênero Candidatus Liberibacter (CL), sendo no
continente Americano transmitida pelo psilídeo Diaphorina citri. Existem relatos
da presença do psilídeo no Brasil desde o ano de 1942, embora sem
17
notificações da doença em citros no período (LIMA, 1942). Os frutos
sintomáticos das laranjeiras infectadas apresentam coloração inadequada, são
pequenos, geralmente amolecidos, possuem forma assimétrica e as suas
características sensoriais têm sido associadas aos atributos negativos referente
ao suco de laranja, incluindo: elevação do amargor, acidez, sabor metálico,
fermentado, salgado/umami, adstringência, redução da doçura e sabor cítrico
(PLOTTO et al., 2008; PLOTTO et al., 2010; DALA PAULA et al., 2017a; 2017b).
Além disso, o HLB pode causar a devastação de grandes plantações e
consequente prejuízo econômico aos agricultores, indústria de alimentos e
exportadores da fruta e seus derivados (BOVÉ, 2006; BASSANEZI et al., 2009;
COSTA, 2011; BALDWIN et al., 2017).
O aroma do suco de laranja se deve à complexa combinação de vários
odores e sabores derivados de seus componentes. Os álcoois, aldeídos,
ésteres, cetonas, hidrocarbonetos e metabólitos secundários, a exemplo dos
compostos fenólicos e dos limonoides amargos (limonina e nomilina) têm sido
amplamente investigados em suco de laranjas acometidas pelo HLB (PLOTTO
et al., 2008; 2010; BALDWIN et al., 2010; DAGULO et al., 2010; SLISZ et al.,
2012; MASSENTI et al., 2016). Porém, as causas do típico armargor em suco de
laranja acometidas pelo HLB ainda não foram completamente elucidadas. Os
artigos disponíveis na literatura científica relacionam a limonina e a nomilina
como os principais compostos responsáveis pelo amargor, sendo que em alguns
desses estudos, os teores desses metabólitos em suco de laranja acometidas
pelo HLB estavam abaixo do limiar para a sua percepção, entretanto a análise
sensorial indicou percepção do sabor amargo nas amostras estudadas
(BALDWIN et al., 2010; DAGULO et al., 2010; DEA et al., 2013).
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REVISÃO DA LITERATURA
1. CLASSIFICAÇÃO TAXONÔMICA DA LARANJA E PRINCIPAIS
CULTIVARES PLANTADAS NO BRASIL
As frutas cítricas de maior relevância comercial no mundo são do gênero
Citrus, pertencentes à família Rutaceae. Nesse gênero estão incluídas as
laranjas doces, tangerinas, laranjas azedas, pomelos, toranjas, limas ácidas,
limas doces, limões, cidras e outros tipos incluindo híbridos naturais (EMBRAPA,
1998). A classificação taxonômica desse gênero é complexa devido ao elevado
grau de hibridação ocorrido, e ainda, as laranjeiras amargas apresentam
características botânicas semelhantes às das laranjeiras doces (MATTOLI et al.,
2005). Existem algumas divergências em sua classificação, no esquema
taxonômico mais tradicional reconhecido por Swingle e Reece (1967), a laranja
doce é classificada como Citrus sinensis (L.) Osbeck, como uma espécie
separada. Mas em uma classificação mais recente, de acordo com Penso
(1997), laranjas amargas e doces são consideradas como subespécies ou
cultivares Citrus aurantium L. (Rutaceae). Essas são denominadas
respectivamente, C. aurantium L. var. amara e C. aurantium L. var. sinensis
(MATTOLI et al., 2005). Tendo em vista o predomínio da classificação
taxonômica das laranjas, proposta por Swingle e Reece (1967), nos artigos da
área de Ciência de Alimentos, esta também será empregada no presente
estudo.
As laranjeiras são árvores de porte médio e copa esférica, podem ser
classificadas em função do fruto em quatro subgrupos: comum, do grupo Navel
ou laranjeiras de umbigo, sanguíneas e as de baixa acidez. As cultivares
representantes de cada um dos quatro sub-grupos podem apresentar
especificidades quanto à maturação, podendo ser precoce, meia-estação ou
tardia. As principais cultivares plantadas e comercializadas no Brasil estão
representadas na Tabela 1. Pera Rio, Valência, Hamlin, Natal, Valência Folha
Murcha e Valência Americana são as principais cultivares plantadas e
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destinadas ao processamento do suco (CAPUTO, 2012; EMBRAPA, 2014,
FUNDECITRUS, 2017).
Tabela 1. Características das principais cultivares de laranjas plantadas no Brasil
Cultivar
Planta Fruto
Mercado Porte* Copa Maturação Semente Teor de
suco
Acidez
Pera Rio médio ereta A.T. ausente alto baixa I.M.
Valência alto arredondada tardia ausente alto média I.M.
Natal alto compacta tardia ausente alto média I.M.
Folha murcha médio arredondada tardia ausente alto baixa I.M.
Hamlin médio arredondada precoce presente baixo alta I.M.
Bahia alto arredondada M.E. ausente baixo média mesa
Baianinha alto arredondada M.E. ausente baixo média mesa
Lima médio arredondada M.E. ausente baixo baixa mesa
Rubi alto arredondada precoce ausente médio média mesa
Westin baixo semiereta M.E. ausente médio média mesa
*são consideradas de porte alto cultivares acima de 5,0 m; de porte baixo, menores de 1,5 m e de porte médio, entre essas duas medidas. Leg.: A.T.: ano todo; I.M.: indústria e mesa; M.E.: meia-estação. Fonte: EMBRAPA, 2014.
Para atender ao mercado que se destinam (indústria ou consumo in
natura), as laranjas devem apresentar determinadas características, tais como:
intensa e uniforme coloração da casca, ausência ou reduzida quantidade de
sementes, epicarpo ou casca com espessura fina, redimento de suco superior a
35 mL.100 g-1, teores de sólidos solúveis (SS) aproximados à 10 °Brix, faixa de
acidez entre 0,5 e 1,0 g.100 mL-1, destacando que para o consumo in natura o
ratio deve ser acima de 14 e para a produção de suco, acima de 8. As laranjas
de mesa ou consumidas in natura podem ser subdivididas em três grupos
confome a acidez, incluindo: laranjas de baixa acidez, entre 0,005 e 0,1 g.100
mL-1 (Lima e Piralima); laranjas-de-umbigo, com acidez entre 0,92 e 0,94 g.100
mL-1 (Bahia e Baianinha); e laranja comum, aquelas que possuem 0,95 a 1,0
g.100 mL-1 de acidez (Pera Rio, Natal, Folha Murcha e Valência) (EMBRAPA,
2014).
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2. BREVE HISTÓRICO DO CULTIVO E PRODUÇÃO DE LARANJA
A laranja é originária do sudeste da Ásia. A subespécie doce é
amplamente cultivada no mundo, enquanto a amarga é principalmente produzida
em determinadas regiões, como na Espanha (Sevilha e Málaga), Itália (Sicília),
Líbia (Trípoli) e Malta. A laranjeira amarga do norte da Índia parece ter sido
introduzida na África Oriental, Arábia e Síria, de onde os árabes, a partir das
Cruzadas, trouxeram para a Europa em meados de 1200 anos DC. No Brasil, há
evidências de que a laranja doce foi introduzida na Bahia pelas primeiras
expedições colonizadoras. Um fato que reforça a hipótese é a presença da fruta
ao longo do litoral brasileiro desde meados do século XVI (MATTOLI et al.,
2005).
O cultivo de laranjas em grande escala teve início aproximado em 1950
em Limeira, São Paulo, e na década seguinte a citricultura expandiu para as
cidades de Bebedouro e Araraquara, ambas também localizadas no estado de
São Paulo (TOLEDO & CASTILLO, 2008). Ao analisar a produção nacional de
laranjas ao longo dos últimos oito anos (2010-2017), percebe-se uma contínua
redução a partir de 2012. A estimativa da produção de laranjas determinada pelo
Sistema IBGE de Recuperação Automática (SIDRA) em maio de 2017 para a
safra do ano corrente foi de 14.673.412 t (Tabela 2). Caso a estimativa se
concretize, o valor da produção será 7,8% inferior à safra de 2016
(15.917.673 t). A produção de laranjas em 2016 apresentou uma redução de
19,6% e 4,9% em relação à 2011 (19.811.064 t) e 2015 (16.746.247 t),
respectivamente (Tabela 2). O elevado estoque de suco, nacional e
internacional, a crise econômica europeia e mundial, os bloqueios alfandegários
nos EUA a partir de 2012, além do longo período de depreciação nos preços da
laranja configuraram-se como importantes fatores de desestímulo à produção
citrícola nos anos de 2013 e 2014, principalmente. Além dos fatores
mencionados, em São Paulo, no Triângulo Mineiro e no Norte e Nordeste do
Paraná, persistem os problemas fitossanitários como a Clorose Variegada dos
Citros (CVC), a pinta-preta, a leprose, o cancro cítrico e principalmente a doença
HLB, com consequente impacto negativo na produção de laranjas. Dessa forma,
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além da produção de laranjas, a área a ser colhida e o rendimento médio por
hectare também vem apresentando reduções a partir de 2012 (IBGE, 2013).
Dentre os 43 produtos cultiváveis presentes no Levantamento Sistemático da
Produção Agrícola realizado pelo IBGE/SIDRA (2017), distribuídos entre cereais,
leguminosas, oleaginosas, frutas e legumes em geral, a área destinada ao
cultivo da laranja foi equivalente a cerca de 0,93% da área total destinada ao
cultivo dos produtos listados (IBGE/SIDRA, 2017).
Tabela 2. Área destinada à colheita de laranja em hectares e quantidade produzida em mil toneladas no Brasil, durante os anos de 2010 a 2017*.
Local Área destinada à colheita (hectares)
2010 2011 2012 2013 2014 2015 2016 2017
Brasil 851.142 818.685 762.765 719.360 689.047 668.189 741.133 738.658
SP 605.432 563.952 500.549 456.818 430.906 412.861 471.200 457.453
MG 33.092 33.000 36.610 39.567 42.951 44.071 47.082 40.672
Quantidade produzida (mil toneladas)
Brasil 18.503 19.811 18.013 17.549 16.928 16.746 15.918 14.673
SP 14.269 15.293 13.366 13.019 12.291 12.279 11.628 10.296
MG 817 824 864 894 940 987 961 900
*os números são referentes às safras iniciada no ano em questão com término no início do ano seguinte. Leg.: SP: São Paulo, MG: Minas Gerais. Fonte: IBGE/SIDRA, 2015 e IBGE/SIDRA, 2017 (adaptado).
Em 2016, os produtores brasileiros sentiram-se encorajados a expandir
seus investimentos nos pomares, devido ao repentino aumento no preço da
caixa de laranja (IBGE, 2017). Ainda hoje, o estado de São Paulo é considerado
o de maior importância para o cultivo da fruta. Em 2016, São Paulo contribuiu
com 73,1% do total de laranjas colhidas no país, sendo sua safra equivalente a
11.628.150 t. Conforme tendência nacional, o estado de São Paulo também
apresentou um declínio da produção estimada para o ano de 2017, assim como
na contribuição do total colhido no país, sendo previsto o percentual de 70,6%
da safra de 2017 (IBGE, 2017).
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As áreas plantadas com laranjas no Brasil e em especial no estado de
São Paulo sofreram consecutivas reduções e mudanças no perfil do produtor.
Em 2017 a previsão da área destinada ao cultivo de laranja foi de
aproximadamente 457 mil hectares, correspondente à 75,6% da área registrada
em 2010 (IBGE, 2017). Apesar da tendência de redução das áreas destinadas à
colheita, em 2016 foi registrado um aumento de 14% em relação a 2015 (Tabela
2).
Os pomares com dimensões menores estão perdendo espaço e
geralmente acabam absorvidos pelo cultivo da cana-de-açúcar. Isso devido às
desleais condições de competição entre os pequenos agricultores e aqueles
inseridos no agronegócio e também pelos problemas fitossanitários. A queda da
produtividade do pequeno produtor o torna pouco competitivo no mercado,
principalmente quando sua atividade é exclusivamente a produção de laranja e
as dificuldades financeiras impedem a renovação do pomar com a formação
moderna dentro dos padrões que garantam alta produtividade. Com este
comportamento, a citricultura brasileira, que tradicionalmente era composta de
pequenos produtores, está mudando o perfil, diminuindo consideravelmente o
número de produtores, ao mesmo tempo em que o cultivo em maiores áreas
torna-se mais expressivo. Assim, 1% (251) dos produtores que produziam 45%
da laranja passou a produzir mais de 60% no estado de São Paulo. O aumento
na participação se deu pelo estabelecimento dos novos plantios, a maioria de
forma adensada, onde o maior número de pés de laranja por unidade de área
tem aumentado a produtividade (CONAB, 2011).
O estado de Minas Gerais, representado especialmente pelo triângulo
mineiro vem aumentando sua área destinada à colheita da fruta, embora ainda
represente aproximadamente 9 a 10% da área destinada à colheita da laranja
pelo estado de São Paulo. Minas Gerais apresentou um aumento da produção
de laranjas ao longo de 2011 a 2015. Após esse período, registrou-se uma
consecutiva queda em sua produção (Tabela 2) (IBGE, 2017).
A citricultura brasileira é considerada uma atividade moderadamente
rentável em longo prazo, mas que envolve consideráveis riscos: de mercado, de
insumos, de produto e os riscos climáticos. Assim a citricultura tem sua
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produção influenciada por inúmeros fatores, tais como: genótipo da laranja, solo,
idade do pomar, pragas, doenças e manejo cultural. Todos esses fatores
interferem na rentabilidade do negócio de citros, pois afetam custos e receitas,
fazendo-os divergir do esperado pelos produtores. Para essa atividade no Brasil,
a principal fonte de risco é a perda de produtividade causada pelo ataque de
pragas e doenças, principalmente o HLB. As condições climáticas também são
fundamentais, visto que são determinantes no desenvolvimento de inúmeras
doenças, assim como no processo fisiológico de desenvolvimento dos frutos. As
condições climáticas correspondem a fatores de riscos mais acentuados para o
estado da Flórida, nos EUA, uma vez que a região é alvo constante de
tempestades tropicais e furacões. Essa percepção do risco se deve ao fato de
que ao longo da história, a cultura de laranja foi constantemente atacada por
pragas e doenças, sendo que, atualmente, considera-se que existam 300 pragas
e doenças afetando a citricultura paulista (ADAMI, 2010).
3. OCORRÊNCIA E EFEITO DA HUANGLONGBING NOS POMARES DE
LARANJA
Nesse tópico serão aborados os aspectos econômicos envolvidos com a
presença do HLB em pomares de laranjas, enquanto no Capítulo II serão
apresentados os agentes causadores e vetores, a incidência dos mesmos e do
HLB ao redor do mundo, os efeitos da doença nos parâmetros físico-químicos,
composição química e característica sensoriais de laranjas e de seu suco, assim
como nas folhas, raízes e em suas árvores. O HLB é uma doença de difícil
manejo devido ao prolongado período de latência da bactéria Candidatus
Liberibacter asiaticus (CLas) na árvore, distribuição irregular do patógeno na
planta, efeitos do ambiente (em especial da temperatura) sobre a expressão dos
sintomas e, possivelmente, sobre a multiplicação da bactéria e variações
potenciais de resistência à bactéria tanto pelas espécies cítricas quanto pelo
inseto vetor.
A tentativa do controle da doença tem sido realizada, principalmente, a
partir do emprego de mudas sadias produzidas em ambiente protegido do
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contato com o psilídio, vetor da doença, da erradicação das árvores doentes e
do controle químico do vetor. Dessa forma, com o controle químico tem-se
aumentado a utilização de inseticidas em pomares, causando sérios impactos
ambientais, econômicos, sociais e na saúde dos trabalhadores rurais e dos
consumidores, o que sugere a insustentabilidade dessa prática (BOVÉ, 2006;
GOTTWALD et al., 2012). Os impactos sociais também podem ser percebidos
devido às mudanças no sistema de produção e também à substituição dos
pomares de laranjas por outras culturas que não requerem trabalho intensivo
como a produção de frutas (MIRANDA et al., 2012). O HLB pode matar ou
debilitar uma árvore cítrica em dois a dez anos, sendo que ainda hoje não
existem métodos curativos eficazes para a doença que possam ser usados em
pomares comerciais, permitindo assim que a fitopatologia cause grande
devastação da cultura (BASSANEZI et al., 2009; BALDWIN et al., 2010).
O HLB foi reportado pela primeira vez no sul da China em 1919 e
atualmente sabe-se que está presente em 50 diferentes países da Ásia, África,
Oceania e Américas do Sul, Central e do Norte (CABI, 2017; EPPO, 2017), mas
somente a partir de 2004 surgiu no estado da Flórida, EUA, e no Brasil. Segundo
Costa (2011), enquanto os países da América não possuíam o registro da
doença, o crescimento da produção foi superior ao observado naqueles países
com registros históricos da doença. Com o início da incidência do HLB nos
pomares de citros do Brasil e dos EUA, verificou-se uma retração na taxa de
crescimento anual para o período de 2000 a 2008 da produção dos países das
Américas. Concomitantemente, houve aumento na taxa anual de crescimento
da produção de alguns países africanos e asiáticos, principalmente China e
Indonésia.
Segundo Miranda et al. (2012), o estado de São Paulo (SP) tem
enfrentado um aumento da incidência do HLB, o que coloca em risco a
sustentabilidade da produção de laranjas. No Brasil, a doença foi relatada pela
primeira vez em março de 2004, em Araraquara, na região central de SP. Mais
tarde, em outubro de 2004, a infecção havtia alcançado em média 3,4% dos
blocos de pomares no estado. Consideraram-se como pomares comerciais,
aqueles com população de duzentas ou mais plantas cítricas, da mesma
B
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espécie, idade, sob os mesmos tratos culturais, plantadas no mesmo
espaçamento e sem ruas ou corredores que dividam o bloco de plantas. Em
2010, a amostragem do FUNDECITRUS indicou 38,8% de blocos com pelo
menos uma planta sintomática e 1,9% de árvores infectadas em SP. No último
levantamento, em agosto de 2011, os blocos e as árvores infectadas haviam
atingido, respectivamente, 53,4 e 3,78%.
Em SP, as ações de defesa sanitária vegetal para o controle da doença
vêm sendo executadas pela Coordenadoria de Defesa Agropecuária (CDA) em
conjunto com o Ministério da Agricultura, Pecuária e Abastecimento (MAPA) e a
Agência Paulista de Tecnologia dos Agronegócios (APTA). Cerca de um ano
após a primeira constatação do HLB no Brasil, foi publicada a Instrução
Normativa/MAPA nº 10, de 2005, posteriormente substituída pela Instrução
Normativa/MAPA nº 32, de 2006, que determinou a eliminação de plantas
cítricas sintomáticas e comprovadamente infectadas pelas bactérias causadoras
do HLB. Atualmente, está em vigor a Instrução Normativa/MAPA nº 53, de 2008,
que garante uma maior agilidade no processo de fiscalização, atribuindo novos
deveres a todos os produtores de citros, como a elaboração de um relatório
semestral informando a incidência do HLB nas fazendas e determinando a
eliminação de plantas sintomáticas e assintomáticas do mesmo talhão1, quando
a incidência da doença for superior a 28%. Houve ainda a publicação da Portaria
CDA-21, de 15/12/2011, na qual todo o estado de SP fica delimitado e
oficializado como área sob vigilância fitossanitária visando o controle do HLB
(MAPA, 2005; MAPA, 2006; MAPA, 2008; RUIZ et al., 2010; CDA, 2011).
O sucesso do controle do HLB depende da ação conjunta de todos os
citricultores. Desse modo as ações governamentais que objetivam eliminar as
fontes de inóculos oriundas de propriedades que não cumprem a legislação
específica para a doença, são justificadas, pois se não forem feitas, podem
colocar em risco a sanidade dos pomares das propriedades circunvizinhas
(RUIZ et al., 2010). No entanto, o prejuízo associado à eliminação das
laranjeiras sintomáticas ou mesmo de toda a cultura tem desestimulado muitos
1 Talhão: fração ou parcela de uma propriedade separada por ruas, estradas, carreadores ou outro meio qualquer, geralmente, com largura superior ao espaçamento entre linhas (FUNDECITRUS, 2017).
26
citricultores em atender a Instrução Normativa/MAPA nº 53, de 2008. Essa ação
compromete o controle do HLB pelo risco de deslocamento da doença para
outros pomares vizinhos onde a doença não foi diagnosticada e regiões
brasileiras ainda livres (MAPA, 2008; MIRANDA et al., 2012).
Além da incidência do HLB, outros fatores também contribuíram para o
aumento dos custos da produção e distribuição de laranjas. Os custos de
colheita e transporte da fruta até as fábricas sofreram impactos relevantes no
período entre as safras de 2003/2004 e 2009/2010. A média dos custos
operacionais de produção da laranja dos pomares próprios das indústrias
colocadas no portão das fábricas para esse intervalo de tempo sofreu um
acréscimo, em dólares, de 202%. O custo saltou de US$ 1,31 para US$ 3,96 por
caixa de 40,8 Kg. Nesses cálculos estão inclusos os custos de colheita e
transporte dos frutos, porém, está excluído o cálculo de depreciação e
amortização do capital investido. Contribuiu também para a escalada dos custos
agrícolas, uma forte inflação de custos de mão de obra, insumos agrícolas e
incremento de tratamentos fitossanitários contra o cancro cítrico, HLB e pinta
preta (NEVES et al., 2009).
4. BREVE HISTÓRICO DA PRODUÇÃO DE SUCO DE LARANJAS
O sucesso da produção nacional de laranjas pode ser explicado pelas
excelentes condições climáticas do Brasil para o cultivo da fruta, assim como
pela instalação das grandes indústrias de suco concentrado na região Sudeste
do país, em especial, no estado de SP em meados da década de 60. Estas
proporcionaram o desenvolvimento do maior parque citrícola do mundo, que,
desde a sua criação, teve como principal escoamento de produção o mercado
internacional (TOLEDO & CASTILLO, 2008).
Desde 1962, quando começaram as primeiras exportações, a citricultura
tem contribuído de forma definitiva para o desenvolvimento do Brasil. Em 2009,
as exportações do complexo citros somaram 2,9 milhões t, sendo 1,129 milhão t
de suco de laranja concentrado e congelado (do inglês Frozen Concentrated
Orange Juice - FCOJ), 939 mil t de suco de laranja não concentrado (do inglês
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Not from Concentrate Juice - NFC), e 851 mil t de subprodutos (NEVES et al.,
2009). Em 2014 o Brasil produziu 1,831 milhão t de suco de laranja, no entanto,
apresentou uma redução de aproximadamente 12,1% de sua produção quando
comparado a 2013, cuja produção foi de 2,084 milhões t (CONAB, 2017). A safra
que se iniciou em 2015 gerou uma das piores quedas de produtividade de FCOJ
já registrada na história da citricultura paulista – cerca de 25,7% menor que o
equivalente obtido na safra iniciada em 2014. Uma das principais causas
naturais levantadas para o ocorrido foi o aumento, acima da média, das chuvas
em decorrência do fenômeno El Niño durante os principais meses de colheita.
As consequências afetaram diretamente as indústrias de suco de laranja uma
vez que recebeu sua matéria prima com reduzido percentual de suco na fruta,
aumento do percentual de casca e polpa e redução do teor de SS de 12 °Brix na
safra 2014 para 10,2 °Brix na safra de 2015 (CITRUSBR, 2016a). Ainda,
segundo os dados da Associação Nacional dos Exportadores de Sucos Cítricos
(CITRUSBR, 2016b) fornecidos ao Fundo de Defesa da Citricultura
(Fundecitrus), a produção de suco de laranja provenientes da safra de 2015
(finalizada em abril de 2016) pelos produtores associados ao CitrusBR no
Cinturão Citrícola Paulista e Triângulo Mineiro foi de 795.463 t FCOJ.
Considerando o mesmo rendimento industrial médio aplicado das indústrias
associadas ao CitrusBR aos processadores não associados, pode-se inferir uma
produção aproximada de 70.000 toneladas de FCOJ. Esses números foram
maiores que aqueles apresentados recentemente para a safra de 2016
(finalizada em abril de 2017). A produção de FCOJ pelos produtores associados
ao CitrusBR do Cinturão Cintrícola Paulista e Triângulo Mineiro foi de 648.004 t,
já para os não associados foi de aproximadamente 54.000 t (CITRUSBR, 2017).
A citricultura norte-americana ocupa a quarta posição mundial em volume
de produção do fruto, sendo o estado da Flórida a grande região produtora.
Entretanto, diferentemente do Brasil, a maior parte da produção americana é
destinada ao abastecimento do mercado interno, e não à exportação. O impacto
da safra americana na exportação do suco brasileiro se deve ao fato do Brasil
ficar na dependência dos resultados da produtividade dos pomares da Flórida,
para que os EUA comprem o suco brasileiro, com o objetivo de suprir a
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demanda interna. Caso a produção americana seja suficiente para o seu
abastecimento, as indústrias brasileiras ficam com grande quantidade de suco
sem um mercado certo para exportação, gerando um estoque ocioso,
impulsionando assim a queda do preço do produto. Para se tornarem menos
suscetíveis à influência americana, os citricultores brasileiros vêm buscando
maior diversificação no mercado.
A citricultura brasileira conseguiu uma boa eficiência na cadeia citrícola.
Desde mudas e viveiros certificados, plantio e cultivo da laranja, produção do
suco de laranja até a distribuição internacional em sistemas integrados a granel
com caminhões-tanques, terminais portuários e navios dedicados que levam ao
consumidor europeu, norte-americano e asiático produtos citrícolas com
dezenas de especificações e misturas (blends) para as mais variadas
aplicações. Além disso, é responsável por cerca de metade do suco de laranja
do planeta cujas exportações trazem de US$ 1,5 bilhão a US$ 2,5 bilhões por
ano ao país. Grande parcela do suco distribuído é feito por empresas
multiprodutos, nas quais o suco de laranja integral corresponde a apenas mais
um item de seu vasto portfólio de bebidas, como néctares e refrescos de outros
sabores, água, refrigerantes, energéticos, lácteos e demais bebidas não
alcoólicas, que invariavelmente canalizam mais investimentos de marketing.
Estas empresas dão mais atenção e prioridade de produção àquelas categorias
de bebidas que estão em alta e oferecerem maior margem de lucro, mesmo
sendo algumas dessas de qualidade nutricional inferior ao suco integral de
laranja (NEVES et al., 2009).
Com o mercado altamente competitivo, as indústrias de bebidas apostam
na diversificação de sua linha de produtos. Além do suco (concentrado, integral
e reconstituído), o néctar é outra opção de bebida à base de laranja. Por possuir
menor teor de suco (ingrediente de maior custo), o preço final dos néctares é
menor que os preços praticados de sucos integrais e sucos reconstituídos.
Neste aspecto, os néctares vêm ganhando espaço entre os consumidores
(FIGUEIRA et al., 2010).
Nas safras, de 1995/96 a 2009/10, a queda na produção mundial de suco
foi de 13% (equivalente a 308 mil toneladas). As maiores reduções aconteceram
29
na Flórida em 295.000 t e no cinturão citrícola de SP e Triângulo Mineiro em
31.000 t. O surgimento do HLB em citros em meados de 2004 no Brasil e 2005
nos EUA possivelmente contribuiu com a diminuição da produção de suco de
laranja. Apesar da queda notificada, essas regiões continuam liderando a
produção mundial de suco de laranja, com 81% de toda a produção (NEVES et
al., 2009).
5. ETAPAS DO PROCESSAMENTO E COMERCIALIZAÇÃO DO SUCO DE
LARANJA PRODUZIDO NO BRASIL
A laranja é considerada uma fruta de padrão de maturação não-
climatérica, assim como os demais citros. Não há incremento na produção de
etileno ou na taxa de respiração associado com a maturação. Assim, para o
processamento do suco de laranja, essa deve ser colhida após a maturidade
fisiológica e quando o produto apresentar as características de qualidade
adequadas para o consumo ou para a comercialização (CHITARRA &
CHITARRA, 2005).
O processo de produção de FCOJ consiste em várias operações
industriais de grande escala, além do suco, há vários subprodutos obtidos
durante o seu processamento da laranja, conforme ilustrado na Figura 1. Após a
colheita, as laranjas são transportadas, geralmente em caminhões ou carretas,
até o pátio das empresas. Durante o descarregamento dos frutos, uma amostra
representativa da carga é coletada e destinada ao laboratório de controle de
qualidade, a fim de se avaliar a cor, defeitos e extração do suco visando
monitorar o rendimento e o teor de SS, AT e ratio. As laranjas passam por
procesoss de lavagem e sanitização, sem que a superfície da fruta seja
danificada, a higienização usualmente é realizada por um sistema de aspersão
de água quente e clorada, com escovas rotativas. Em seguida as laranjas são
descarregadas em plataformas inclináveis e levadas por meio de esteiras para
as mesas de seleção manual. Durante o trajeto, os frutos que apresentarem
ferimentos nas cascas, que estiverem excessivamente danificados por ácaros ou
contendo sujidades, não apresentarem dimensões adequadas ou apresentarem
30
em estágio avançado de senescência são rejeitados. Os resíduos e os descartes
da seleção dos frutos são pesados e enviados à fábrica de ração para serem
transformados em farelo de polpa cítrica, a partir do processo de secagem da
matéria prima. Será formada uma forragem concentrada que serve de ração
para alimentação animal.
As laranjas sadias são classificadas automaticamente por tamanho a fim
de permitir o ajuste dos copos das extratoras em função do seu tamanho. Os
frutos são transportados por elevadores de canecas aos silos de armazenagem,
onde ficarão até serem encaminhados para a etapa de extração (CETESB,
2005; MACHADO, 2010). A etapa de extração é a principal etapa do processo
de obtenção do suco diretamente da laranja, e tem por finalidade separar o suco
do bagaço, da casca e da semente. Nessa etapa ocorre a separação do suco de
laranja, da emulsão que dará origem ao óleo essencial, do bagaço e da casca
que darão origem à polpa cítrica e da polpa que poderá ser readicionada ao
suco conforme solicitação do cliente. Na indústria de cítricos há várias extratoras
acopladas em série que são projetadas para extrair o máximo de suco, evitando
incorporar componentes da casca e óleo essencial. Geralmente as extratoras de
suco de laranja são formadas por copos que se interpenetram comprimindo a
fruta inteira e separando as frações de interesse comercial (CETESB et al.,
2005; RODRIGUES & FERRI, 2012).
A quantidade de suco extraído da laranja pode variar em uma faixa de 35
a 60 mL.100 g-1 dependendo das condições climáticas, da cultivar, do tamanho
do fruto e das condições de extração. Durante a etapa de extração, ocorre o
rompimento das células de óleo essencial presentes na casca que
posteriormente será recuperado e utilizado na produção de compostos para
bebidas, cosméticos e produtos químicos. O D-limoneno ou terpeno cítrico é o
principal componente do óleo da casca da laranja, sendo utilizado como matéria-
prima para a fabricação de resinas sintéticas e adesivos pelas indústrias de
plásticos (CITRUSBR, data de publicação não informada).
31
Figura 1. Esquema de uma planta de processamento comercial de suco de laranja. Fonte: JBT, 2015 (modificado).
Análise preliminar (SS, AT, ratio)
Recebimento das laranjas
Lavagem com escova
Seleção manual
Classificação das frutas
Armazenamento da fruta nos silos
Extração
Casca
Trituração/prensagem
Membranas e sementes
Secagem
Peletização
Polpa cítrica
Recuperação de Sóidos
Secundários
Fragmentos de casca + emulsão
Filtração/Separação
Centrifugação
Óleo essencial
Suco + Polpa
Filtração/finisher
Centrifugação
Concentração
Homogeneização e resfriamento
FCOJ
Polpa
Pasteurização/
Resfriamento
Fases aquosas e oleosas
Evaporador de
calor residual
D-Limoneno ou
Terpeno cítrico
NFC
32
Após a extração, o suco passa pela etapa de clarificação, uma vez que
ainda contém polpa e resíduos de bagaço que são removidos por centrifugação
ou em equipamentos denominados finishers (despolpadeiras), os quais separam
a polpa do suco por filtração. Este processo consiste numa operação na qual o
suco é tranportado por uma rosca sem fim que aplica uma pressão contra uma
peneira (cuja malha é de 0,64 a 1,27 mm) separando assim os sólidos. Em
geral, o teor de polpa do suco fica em torno de 4%. A polpa pode ser utilizada na
produção de outros produtos, como por exemplo, o suco obtido da polpa (pulp
wash) (RODRIGUES & FERRI, 2012).
Antes do processo de concentração, os sucos são pasteurizados, dessa
forma, ocorre a inativação de micro-organismos responsáveis pela degradação
do suco de laranja e da pectinesterase, enzima responsável pela
desesterificação da pectina, produzindo metanol e pectina com baixo teor de
metoxilação. A pectina com baixo teor de metoxilação pode se ligar a íons de
cálcio presentes e precipitar-se, afetando assim a qualidade do suco. Com isso a
pectina que antes auxiliava na estabilização da turbidez, perde o seu papel,
causando além da redução da turbidez, a alteração do sabor e do aroma
(TRIBESS, 2003; CETESB, 2005; MACHADO, 2010, CITRUSBR, data de
publicação não informada).
A concentração do suco de laranja consiste na extração da água de
constituição do suco, reduzindo assim sua atividade de água. As temperaturas
utilizadas para concentrar o suco são de 90 a 95 ºC, em evaporadores à vácuo
(RODRIGUES & FERRI, 2012). O SS inicial do suco, geralmente na faixa de 10
a 11 °Brix, aumenta ao final do processo para 65 °Brix, padrão de qualidade fo
FCOJ. Em seguida, o concentrado é armazenado a - 6,6 ºC ou temperatura
inferior até que seja envasado para a venda. É possível armazenar o FCOJ
durante vários anos, desde que em temperaturas adequadas. Assim, a utilização
desse método de conservação favorece a produção de suco de laranja
reconstituído. Sendo a via de produção de suco, a partir do reconstituído, a mais
empregada em todo o mundo (VIEIRA et al., 2010).
Do processo de evaporação do suco de laranja pode-se obter a essência,
formada por componentes polares e apolares, dissolvidos em uma fase aquosa
33
e outra oleaginosa. Esse subproduto pode ser readicionado ao suco, assim
como pode ser usado para outros fins nas indústrias de bebidas e alimentos
(CETESB, 2005; CITRUSBR, data de publicação não informada).
A indústria de suco concentrado tem se esforçado para reduzir o volume
de sucos cítricos por eliminação do conteúdo de água. Esta redução é
importante por duas razões principais, primeiro, por facilitar o transporte
marítimo reduzindo o tamanho dos containers. Em segundo lugar, por ser
vantajoso do ponto de vista de conservação, possibilitando o seu consumo fora
do período de colheita. A especificação FCOJ se refere ao suco de laranja com
teor de SS igual ou superior a 42,0 °Brix (VIEIRA, 2006; FLORIDA
DEPARTMENT OF AGRICULTURE AND CONSUMER SERVICES, 2016).
O suco de laranja originário do Brasil é conhecido por sua elevada
qualidade; além disso, o país é o maior produtor e exportador mundial de FCOJ.
O volume de FCOJ exportado pelo Brasil no período de 2014 a 2016, a partir do
porto de Santos, apresentou um discreto aumento de 4,17%, sendo o volume de
exportação em 2016 equivalente a 1.080.448 t. No entanto, a exportação de
FCOJ durante os meses de janeiro a abril de 2017 sofreu uma queda
considerável quando comparado com o ano anterior (Figura 2).
Para produzir o FCOJ exportado em 2014, 2015 e 2016 as indústrias
processadoras de suco do Cinturão Citrícola Brasileiro utilizaram
aproximadamente 83%, 87% e 86%, respectivamente, do total de laranjas
produzidas no Estado de SP. Esses valores estão próximos à porcentagem
média utilizada entre os anos de 2004 a 2011, equivalente a 88,8%, porém
discrepante da porcentagem utilizada em 2012, equivalente a 79% (FLORIDA
DEPARTMENT OF CITRUS, 2016). Em 2012 o mercado brasileiro de citros
sofreu embargos alfandegários dos EUA, além da redução das vendas à União
Europeia proporcionado por reflexos da crise econômica.
34
0
200000
400000
600000
800000
1000000
1200000
1400000
1600000
Figura 2. Exportações de FCOJ equivalente em toneladas por ano civil a partir do porto de Santos. Leg: *até abril de 2017. Fonte: CITRUSBR, 2016b.
O tipo de suco produzido é estabelecido pelo comportamento do
consumidor em mercados de mais alto poder aquisitivo, que nos últimos anos
passou a preferir o NFC ao FCOJ, por ser um produto de paladar mais
agradável, com sabor mais aproximado ao suco extraído na hora e por ter a
imagem de uma bebida mais saudável. As primeiras produções de NFC no
Brasil começaram em 1999/2000 ainda em caráter experimental, e em 2000
foram realizadas as primeiras exportações (NEVES et al., 2009).
O volume de NFC exportado pelo Brasil tem aumentando continuamente
ao longo dos anos, com destaque para 2016, que ultrapassou a quantidade de
1,4 milhões de toneladas (CITRUSBR, 2016b). Assim como o FCOJ, as
exportações para os meses de janeiro a abril de 2017 foram inferiores ao do
mesmo período de 2016 (Figura 3).
35
0
200000
400000
600000
800000
1000000
1200000
1400000
1600000
Figura 3. Exportações de NFC equivalente em toneladas por ano civil a partir do porto de Santos. Fonte: CITRUSBR, 2016b.
6. CONSUMO DA LARANJA IN NATURA E SEUS DERIVADOS
O consumo interno da laranja in natura é crescente e recebe apoio a partir
da prática comum do preparo de suco nas residências, em padarias e
restaurantes, além do mercado de suco pasteurizado produzido em fábricas com
atuação regional. Uma laranja média pode gerar cerca de 90 g de suco. O
mercado doméstico de laranja in natura se tornou um grande consumidor da
produção brasileira uma vez que mais de 100 milhões de caixas de laranja (40,8
kg/caixa), equivalente a aproximadamente 30% da produção nacional, são
consumidas pelo povo brasileiro que tem à sua disposição uma fruta nutritiva a
um preço competitivo (NEVES et al., 2009; NEVES & TROMBIN, 2011).
O suco de laranja é um produto de grande importância econômica para as
exportações brasileiras. O agradável sabor, além das atrativas propriedades
nutricionais torna essa bebida muito apreciada e consumida por populações de
36
diferentes culturas e hábitos alimentares. Dentre os sucos de frutas, o de sabor
laranja é o mais consumido no mundo. Em 2016, o consumo de suco integral de
laranja representou 45% dentre o total de sucos de frutas consumidos pelos 40
principais países que representam 99% do consumo mundial da bebida
(MARKETSTRAT, 2016). Apesar do destaque do suco integral de laranja dentre
os demais sabores, o seu consumo em nível mundial vem apresentando
redução ao longo dos anos. Para o período compreendendo entre 2003 a 2015,
a redução foi equivalente a 2.608 milhões de litros. Os sete principais
consumidores mundias de suco de laranja são: EUA, Alemanha, França, China,
Canadá, Reino Unido e Brasil.
A situação de mercado para o FCOJ não é diferente daquela do NFC.
Analisando o período de 2003 a 2015, o consumo reduziu 19,4%, sendo os
EUA, Alemanha, França, China e Canadá os países responsáveis pelas quedas
mais expressivas. Em 2015 o consumo aproximado de FCOJ pelos EUA foi
equivalente a 613.000 t e no Brasil, 63.000 t (CITRUSBR, 2016a;
MARKETSTRAT, 2016).
Em 2010 alguns fatos surgiram como promessa de melhoria para o
mercado mundial de FCOJ. O consumo durante o ano de 2010 voltou a crescer
na média de 1% em comparação ao de 2009. O incremento desse consumo foi
observado nos países emergentes, ainda com mercado pequeno, mas também
houve recuperação em alguns mercados tradicionais europeus. Em apenas um
ano, estes consumiram 42 mil t a mais de FCOJ. A soma destes crescimentos
em 2010 compensou a queda observada nos EUA (NEVES & TROMBIN, 2011).
No entanto, o ano de 2013 refletiu as perdas na citricultura paulista, verificadas
em 2012. A redução do fluxo dos estoques de suco dificultou a comercialização
das frutas e até mesmo o seu apodrecimento nos pomares. A crise no Mercado
Europeu e as barreiras alfandegárias impostas pelos EUA foram consideradas
as principais responsáveis pelos prejuízos à citricultura brasileira no ano de
2013. A safra nacional, de 400,6 milhões de caixas, apresentou decréscimo de
14,6%, em relação à safra colhida em 2012. A laranja para indústria, em SP,
fechou o mês de setembro de 2013 com o preço da caixa de laranja sendo
comercializada a R$ 7,66, considerado baixo pelos produtores (IBGE, 2013). Em
37
contrapartida, os preços atuais (fevereiro e março de 2017) recebidos pelos
produtores tiveram aumento de 107,4% em SP, 60,0% em Minas Gerais e
197,4% na Bahia, se compardos ao relativo mês de fevereiro de 2016. Segundo
os dados da conjuntura mensal para a produção da laranja Pera Rio publicados
pela Companhia Nacional de Abastecimento (CONAB), em fevereiro de 2017, os
preços recebidos pelos produtores por uma caixa de laranja nos seguintes
estados foram: SP (R$ 30,96), Minas Gerais (R$ 24,00) e Bahia (R$ 23,05).
Sendo o preço no atacado equivalente a: R$ 79,97; R$ 75,07 e R$ 31,82,
respectivamente, para os estados citados anteriormente (CONAB, 2017).
7. COMPOSIÇÃO QUÍMICA E NUTRICIONAL DO SUCO DE LARANJA
Os principais componentes do suco natural de laranja são os
carboidratos, que constituem mais de 70% dos SS. Em segundo lugar são os
ácidos orgânicos, principalmente o cítrico e o málico, que representam até 10%
dos SS. O restante é composto por aminoácidos livres, bases nitrogenadas
(6%), íons inorgânicos (aproximadamente 3%), vitaminas (2,5%), lipídeos (1,2%)
(Tabela 3), flavonoides (1,2%) e outros (VIEIRA, 2006; VIEIRA et al., 2010;
TACO, 2011).
Aproximadamente 70% dos compostos nitrogenados são aminoácidos
livres e o restante do nitrogênio encontra-se na forma de proteínas, enzimas,
aminas, nucleotídeos, ácidos nucleicos, fosfolipídios e vitaminas. A prolina é o
aminoácido predominante no suco de laranja, representando 50% do total de
aminoácidos livres (VIEIRA, 2006). Slisz et al. (2012) identificaram os principais
aminoácidos presentes no suco de laranja: alanina, arginina, asparagina,
aspartato, histidina, isoleucina, leucina, fenilalanina, prolina, treonina e valina,
com prevalência da prolina, seguida pela arginina, asparagina, aspartato e
alanina. O teor calórico da fruta in natura é proveniente em 90% dos
carboidratos, 6% da proteína e 4% dos lipídeos, enquanto no suco, os
carboidratos representam 92% do teor calórico total, seguido de 5.5 % das
proteínas e 2.5 % dos lipídeos.
38
Tabela 3. Composição química representativa da laranja Valência in natura e do seu suco.
Os citros contêm uma gama de flavonoides, em especial os compostos
pertencentes ao grupo das flavanonas, geralmente glicosilados por um
disscarídeo no carbono de posição 7. As flavanonas são encontradas em alta
concentrações nas frutas cítricas quando comparadas aos outros vegetais, um
litro de suco de laranja pode conter entre 200 a 600 mg de hesperidina, 15 a 85
mg de narirutina (MANACH et al., 2004) e 8 a 30 mg de didimina (GATTUSO et
al., 2007). Um simples copo de suco de larnaja pode conter entre 40 a 140 mg
de flavanonas glicosiladas (MANACH et al., 2004). A Tabela 4 contém a
concentração média de algumas flavononas, flavonas e flavonas metoxiladas em
laranja Valência, assim como em sua casca e vesículas de suco. As estruturas
Componentes Fruta (por 100 g) Suco (por 100 g)
Calorias (Kcal) 46 37
Proteínas (g) 0,8 0,5
Lipídeos (g) 0,2 0,1
Carboidratos (g) 11,7 8,6
Fibra alimentar (g) 1,7 0,4
Magnésio (mg) 14 10
Cálcio (mg) 34 9
Manganês (mg) 0,06 0,03
Fósforo (mg) 20 17
Ferro (mg) 0,1 Tr
Potássio (mg) 158 143
Cobre (mg) 0,04 0,04
Tiamina (mg) 0,07 Tr
Riboflavina (mg) 0,04 Tr
Piridoxina (mg) 0,03 0,03
Vitamina C (mg) 47,8 73,3*
Tr = traços. *valor referente ao suco da laranja Pera Rio, uma vez
que a fonte utilizada não informa o seu teor no suco de laranja
Valência. Fonte: TACO, 2011.
39
químicas dos flavonoides determinados na Tabela 4 estão representadas na
Figura 4 (NOGATA et al., 2006). Além dos flavonoides, a laranja também é fonte
de ácidos hidroxicinâmicos, a exemplo do p-cumárico encontrado em laranjas
numa faixa de 17,8 a 18,1 (PEI et al., 2016) e dos ácidos ferúlico e sinápico
(DALA PAULA et al., 2017a; 2017b). As estruturas químicas dos ácidos
hidroxicinâmicos mencionados estão representadas na Figura 4.
Tabela 4. Teores médios de flavonoides em casca, em vesícula de suco e em laranja Valência
Flavonoides Laranja Casca Vesícula de suco
Flavanonas (mg.100 g-1 peso fresco)*
Eriocitrina 15,9 5,9 19,7
Neoeriocitrina 2,7 0,0 5,5
Narirutina 166 66,5 54,3
Naringina 0,0 0,0 0,0
Hesperidina 962 1410 93,2
Neohesperidina 0,0 0,0 0,0
Neoponcirina 57,1 42,1 2,9
Poncirina 0,0 0,0 0,0
Flavonas (mg.100 g-1 peso fresco)*
Rutina 10,8 0,0 21,6
Isorhoifolina 0,3 1,1 0,0
Rhoifolina 1,5 5,8 0,0
Diosmina 1,4 5,5 0,0
Neodiosmina 7,7 3,0 0,0
Flavonas polimetoxiladas (mg.100 g-1 peso fresco)*
Sinensetina 8,8 34,0 0,0
Nobiletina 5,0 18,1 0,6
Tangeritina 2,2 8,5 0,0
Heptametoxiflavona 0,5 2,0 0,0
*Cada valor se refere a média de quatro replicatas. Fonte: NOGATA et al., 2006.
40
Flavanonas
Eriocitrina (R=rutinose, R1=OH, R2=H)
Neoeriocitrina (R=neohesperidose, R1=OH, R2=H)
Narirutina (R=rutinose, R1=R2=H)
Naringina (R=neohesperidose, R1=R2=H)
Hesperidina (R=rutinose, R1=OH, R2=CH3)
Neohesperidina (R=neohesperidose, R1=OH, R2=CH3)
Neoponcirina (R= rutinose, R1=H, R2=CH3)
Poncirina (R=neohesperidose, R1=H, R2=CH3)
Flavonas
Rutina (R=H, R1=OH. R2=H, R3=O-rutinose)
Isorhoifolina (R=rutinose, R1=R2=R3=H)
Rhoifolina (R=neohesperidose, R1=R2=R3=H)
Diosmina (R=rutinose, R1=OH, R2= CH3, R3=H)
Neodiosmina (R=neohesperidoside, R1=OH, R2=CH3,
R3=H)
Flavonas polimetoxiladas
Sinensetina (R=H, R1=OCH3, R2=H)
Nobiletina (R=R1=OCH3, R2=H)
Tangeretina (R=OME, R1=R2=H)
Heptametoxiflavona (R=R1=R2=OMe)
Ácidos hidroxicinâmicos
Ferúlico (R= CH2=CH2-COOH, R1=H, R2=OH,
R3=OCH3)
Sinápico (R =CH2=CH2-COOH, R1=R3=OCH3,
R2=OH)
p-Cumárico (R=CH2=CH2-COOH, R1=R3=H, R2=OH)
Figura 4. Estruturas química de compostos fenólicos encontrados em laranja. Fonte: NOGATA et al., 2006; BENAVENTE-GARCÍA & CASTILLO, 2008).
R
R1
R2
R3
41
8. PROPRIEDADES FUNCIONAIS DA LARANJA
O consumo do suco de laranja fresco e pasteurizado interfere na
constituição da microbiota intestinal. A administração de ambos os sucos
contribui para o aumento de Lactobacillus spp. e Bifdobacterium spp., reduzindo
a população de enterobactérias. Essa alteração da microbiota, por sua vez,
aumenta a atividade antioxidante intestinal, eleva a produção de ácidos graxos
de cadeia curta, importante substrato energético aos colonócitos, e reduz a
produção de amônia. Dessa forma, fica claro o potencial do consumo do suco de
laranja como alimento prebiótico (DUQUE et al., 2016).
O suco de laranja é considerado de elevado valor benéfico por conter
antioxidantes naturais, dentre eles, ácido ascórbico, carotenoides, poliaminas
(espermina e espermidina), fenilpropanoides e os flavonoides, especialmente a
hesperidina e a naringenina. Estudos epidemiológicos associam o consumo
regular de suco de laranja com a redução dos riscos aos danos oxidativos
ocasionados pelos radicais livres e a diminuição da prevalência de doenças
como os diferentes tipos de câncer, doenças cardiovasculares e neurológicas
(GIL-IZQUIERDO et al., 2002; FRANKE et al., 2005; VIEIRA et al., 2007; 2010;
GALAVERNA et al., 2008;).
Com relação aos carotenoides, o suco de laranja constitui-se em uma rica
fonte, podendo ser encontrado o maior número dessas substâncias quando
comparado aos outros sucos de frutas. Estes apresentam grande diversidade
estrutural, assim como importantes funções para a saúde humana, alguns são
pró-vitamina A (β-caroteno, α-caroteno, β-criptoxantina) e outros tais como a
zeaxantina e a luteína estão associados com a preservação da degeneração
macular e com a diminuição da ocorrência de catarata, ambos relatados com o
avançar da idade (GAMA & SYLOS, 2007). No entanto, é importante observar
que no suco de laranja, os teores de vitamina C, compostos fenólicos e
carotenoides podem variar conforme os procedimentos adotados para a sua
produção. Gil-Izquierdo et al. (2002) pesquisaram a interferência do
processamento industrial e extração do suco de laranja realizado a partir de
diferentes técnicas quanto aos teores de compostos fenólicos e vitamina C no
42
suco da fruta. Os autores observaram que a técnica de extração utilizada
industrialmente contribuiu com o aumento de 22% de compostos fenólicos e
25% quando comparado com a extração manual. Também perceberam que a
pasteurização foi capaz de degradar vários compostos fenólicos. Gama e Sylos
(2007) estudaram a alteração nos teores de pigmentos carotenoides em suco de
laranja Valência após a pasteurização (95 a 105 ºC durante 10 s) e observaram
redução (p < 0,05) nos teores de violaxantina e luteína em 38% e 20%,
respectivamente, e na etapa de concentração do suco houve perda de 17% de
luteína. A β-criptoxantina tornou-se o carotenoide mais concentrado nos sucos
pasteurizados. No entanto, com relação aos teores de β-caroteno, α-caroteno, β-
criptoxantina e zeaxantina, que são considerados importantes compostos ativos
contra a degeneração macular e catarata, os autores não observaram
diminuição significativa após as etapas pasteurização e concentração.
Nas cascas e nos frutos imaturos de laranjas amargas, assim como no
suco de laranja, podem ser encontradas aminas fenólicas, tais como a N-
metiltiramina, a octopamin e a sinefrina. Esta última apresenta grande interesse
farmacológico por ser um agente simpatomimético. A sinefrina possui atividades
relacionadas à vasoconstrição e relaxamento da musculatura brônquica,
podendo ser utilizada como descongestionante das vias superiores. E também
pode interferir no metabolismo humano, sendo responsável pela redução da
massa de gordura em humanos obesos uma vez que estimula a lipólise e
aumenta a taxa metabólica e a oxidação de gordura a partir de uma maior
termogênese (MATTOLI et al., 2005; VIEIRA et al., 2010).
43
OBJETIVOS
O presente trabalho teve como objetivo geral determinar as alterações na
físico-químicas, na composição química e nas características sensoriais
responsáveis pelo típico sabor de laranjas sintomáticas para o HLB.
Os objetivos específicos foram:
i) Investigar a influência da época de colheita em uma mesma safra nas
características físico-químicas, bioquímicas e sensoriais do suco de laranja
Valência;
ii) Realizar uma revisão da literatura científica sobre as alterações físico-
químicas, na composição química e nas características sensoriais de suco de
laranjas acometidas pelo HLB;
iii) Avaliar as características físico-químicas, a composição química e as
características sensoriais dos sucos provenientes de laranjas Valência
sintomáticas para o HLB (laranjas colhidas em árvores infectadas pela bactéria
Candidatus Liberibacter asiaticus); e saudáveis (livres da infecção de bactéria
Candidatus Liberibacter asiaticus).
Cada um destes objetivos específicos foi atendido e apresentado na
forma de capítulos:
I. Influence of harvest time on quality of ‘valencia’ oranges and juice, second
season
II. Effect of Huanglongbing (greening disease) on orange juice quality, a review
III. Active taste compounds in juice made from oranges symptomatic of
Huanglongbing (HLB) greening disease.
44
CAPÍTULO I - INFLUENCE OF HARVEST TIME ON QUALITY OF
‘VALENCIA’ ORANGES AND JUICE, SECOND SEASON
ABSTRACT
Valencia’ oranges were harvested from February to May 2012 in the Indian River
area of Florida, and the effect of harvest time on fruit and juice quality was
investigated. This was a follow-up study to one done in 2007, where the fruit
were harvested from southern Florida from February to June. Peel color became
less green and more orange over the season, and juice content in fruit declined
as the season progressed. For sugars, the solids/acid ratio increased over the
season, and titratable acidity, citric acid, and total ascorbic acid declined.
Phenolic compounds generally increased, whereas they had fluctuated in the
previous study. Limonoids generally increased as the season progressed except
for the bitter compound nomilin which remained steady. Alkaloids increased
throughout the season. Hydroxycinnamates all decreased over the season. The
polyamines spermidine and spermine increased, while putrescine remained
constant. For volatiles, terpenes, aldehydes, esters, and ketones increased
steadily or in the last months of the season. Alcohols (aliphatic and terpene
alcohols) did not change over the harvest season. This study confirms changes
of some chemicals over the harvest season, while other secondary metabolites
are more dependent on the climatic conditions during fruit formation and at
harvest.
KEYWORDS: Flavor. Secondary metabolites. Maturity. Juice content.
Artigo publicado:
BAI, J.; BALDWIN, E.; MCCOLLUM, G.; MANTHEY, J.; PLOTTO, A.; DALA
PAULA, B.M.; GLORIA, M.B.A.; WIDMER, W.; LUZIO, G.; CAMERON, R.;
NARCISO, J. Influence of harvest time on quality of ‘Valencia’ oranges and juice,
second season. Proceedings of the Florida State Horticultural Society, v. 126, p.
232-238, 2013.
45
1. INTRODUCTION
‘Valencia’ is the predominant orange cultivar grown in Florida and is
mainly used for juice. This cultivar has good color and flavor and is favored by
the juice industry. The harvest season for ‘Valencia’ juice oranges is generally a
4-month period (March to June) after they first reach acceptable maturity
(SOULE et al., 1967). There is a gradual decrease in titratable acidity (TA) by
decomposition of citric acid, and a slight increase in soluble solids content
(SSC) and a consistent increase of SSC/TA ratio (CHEN et al., 1990; HUTTON
& LANDSBERG, 2000). Florida maturity indices for oranges harvested between
16 Nov. to 31 July are: SSC ≈ Brix > 8.5%, TA > 0.4%, SSC/TA ratio > 10.25,
and juice content > ~45 mL.100 g-1 (4.5 gal per 1.6-bu box) (RITENOUR et al.,
2004).
Fresh oranges as well as orange juice are popular worldwide for their
flavor and nutrition. Orange flavor is a complex mixture of volatile compounds of
which some 200 have been identified (JOHNSON et al., 1996). The most
important volatiles are esters, aldehydes, and terpenes, followed by alcohols,
ketones, and hydrocarbons (NISPEROS-CARRIEDO & SHAW, 1990; PLOTTO
et al., 2004; 2008; SHAW, 1991).
The health benefits of oranges are linked to the secondary metabolites,
including numerous flavonoids (ROUSEFF, 1980; LEE & AEDIN, 2006;
GATTUSO et al., 2007; TRIPOLI et al., 2007), limonoids (MAIER et al., 1980;
MILLER et al., 1989; GUTHRIE et al., 2000; MANNERS et al., 2003),
hydroxycinnamates (KROON & WILLIAMSON, 1999; MANTHEY &
GROHMANN, 2001) and the polyamines spermine and spermidine
(SANTIAGO-SILVA, LABANCA & GLORIA, 2011). Secondary metabolites in
oranges may also contribute to fruit and juice quality in many ways, influencing
the appearance, the taste as well as the possible health benefits (BALDWIN,
1993). It has been noticed previously that bitterness and the limonin content, a
major bitter compound in oranges, decreased during the harvest season
(MAIER et al., 1980). However, very little attention has been given to the
seasonal changes of other secondary metabolites. Since information is lacking
concerning development of flavor volatiles, nutrients and phytonutrients in citrus
fruit during ripening (BALDWIN, 1993), a follow up to a previous study
46
conducted in 2007 (BAI et al., 2009) was done where ‘Valencia’ oranges were
harvested and evaluated over the season for physical and chemical quality
characteristics.
2. MATERIAL AND METHODS
2.1 Fruit sampling
Fruit were harvested from four trees grown in a commercial orchard
located in the Indian River area of Florida on February, March, April, and May
2012. At each harvest time, 20 fruits were picked from each replicate tree. After
measuring fruit weight and peel color, the fruit were cleaned with JBT Fruit
Cleaner 395 (JBT, Lakeland, FL), juiced using a fresh juicer (JBT Fresh’n
Squeeze) and frozen at -20 °C until analysis.
2.2 Peel color and juice content analysis
Peel color was evaluated using a Minolta Chromameter (Model CR-300,
Minolta, Tokyo, Japan) measuring a* and b* values for red/green and
yellow/blue color, respectively, and expressed as a*/b* ratio. Juice content was
measured and expressed as milliliters per 100 g of fresh fruit.
2.3 Sugar and acid analysis
TA was determined by titrating to pH 8.1 with 0.1 N NaOH using an
autotitrator (Metler Toledo DL50, Daigger & Company, Vernon Hills, IL) and
SSC using a refractometer (Atago RX-5000 α, Tokyo, Japan).
For analysis of individual acids, approximately 40 g of juice was
extracted using 70 mL 80% ethanol solution (BAI et al., 2010). The mixture was
boiled for 15 min, cooled and centrifuged at 10,000 × g for 15 min. The
supernatant was brought to 100 mL with 80% ethanol. Ten milliters of the
solution were then filtered through a C-18 Sep-Pak (Waters/Millipore) followed
by a 0.45 μm Millipore filter (BALDWIN et al., 1991). Organic acids, including
ascorbic acid, were analyzed using an Altech OA 1000 Prevail organic acid
column (Altech Corp., Flemington, NJ) with a flow rate of 0.2 mL.min-1 at 35 °C
and a mobile phase of 0.01 N H2SO4. The injection volume was 20 μL using a
47
Perkin Elmer Series 200 autosampler, a Spectra System P4000 pump and a
Spectra System UV 6000 LP detector (Shimadzu) was used for the analysis.
2.4 Secondary metabolite analysis
For sample preparation, 2 mL juice was added to 11 mL methanol in a
Teflon gasket screw-top test tube and shaken for 18 h with an orbital shaker
(VSOS-4P, Pro Scientific, Oxford, CT) at 120 rpm at 25 °C. The mixtures were
centrifuged at 10,000 × g for 15 min. The total volume of supernatant was
adjusted to 12 mL by methanol. Then 1 mL butanol was added, and the sample
was taken to dryness using a Savant centrifugal evaporator. Methanol (2 mL)
was added, and each sample was vortexed for 2 min. Samples were then
passed through a 0.45 μm PTFE filter. The filter was washed with an additional
1.5 mL methanol, and the total volume was adjusted to 4 mL prior to analysis by
HPLC-MS (BALDWIN et al., 2010).
2.5 Peel oil, pectin and pectinmethylesterase (PME)
Peel oil content was determined by the Bromate Titration Method
(SCOTT & VELDHIUS, 1966) and total pectin, measured as galacturonic acid,
was determined using a microplate reader as described in Bai et al. (2010). For
PME, juice 30 mL per sample was homogenized using a Brinkmann PT 10/35
homogenizer (Swizerland) at speed 4 for 45 s. PME activity was determined
titrimetrically with 0.5% citrus pectin (BAI et al., 2010).
2.6 Volatile analysis
Juice (6 mL) was pipetted into a 20 mL vial, and then the vials were
crimp capped with Teflon/silicone septa. Juice samples were incubated for
30 min at 40 °C. A 2-cm solid phase microextraction (SPME) fiber (50/30 μm
DVB/Carboxen/PDMS; Supelco, Bellefonte, PA) was then exposed to the
headspace for 60 min at 40 °C. After exposure, the SPME fiber was inserted
into the injector of a gas chromatography-mass spectrometry (GC-MS) (Model
6890, Agilent, Santa Clara, CA) to desorb the extract for 15 min at 250 °C. The
GC-MS equipment and settings were described in Bai et al. (2011).
Volatile compounds were identified by comparison of their mass spectra
with library entries (NIST/EPA/NIH Mass Spectral Library, version 2.0d;
48
National Institute of Standards and Technology, Gaithersburg, MD), as well as
by comparing RIs with published RIs (KONDJOYAN & BERDAGUÉ, 1996;
ADAMS, 2007).
2.7 Bioactive amines
The juice samples were centrifuged at 11,180 x g at 4 °C for 20 min and
filtered through 0.45 μm HAWP membranes (Millipore Corp, Milford, MA).
HPLC analysis of the extract was performed by ion pair reverse phase HPLC,
post-column derivatization with o-phtalaldehyde and fluorimetric detection at
340 and 445 nm excitation and emission, respectively (VIEIRA et al., 2010).
2.8 Statistical analysis
SAS Version 9.1 (SAS Institute, Gary, NC) was used to analyze the data,
using analysis of variance (PROC ANOVA). Mean separation was determined
by Tukey’s test at the 5% level.
3. RESULTS AND DISCUSSION
3.1 Peel color and juice content
The a*/b* ratio (a* is a measure of redness/greenness and b* is a
measure of yellowness) serves as an indicator of quantitative development of
orange color (AYERS & TOMES, 1966). A greater a*/b* ratio is a sign of deeper
orange color, and a negative value shows more green than orange. The a*/b*
values increased from February to May, indicating that the fruit did not undergo
re-greening as can often happen later in the season (RITENOUR et al., 2004).
The season ended early (May) however, which eliminated the potential for fruit
re-greening in June (Fig. 1A).
Juice content declined over the season (Fig. 1B), but was above the
Florida orange juice standard of 45 mL.100 g–1 (RITENOUR et al., 2004). The
results are similar to previous results (BAI et al., 2009) although there was no
re-greening in this season.
49
Figure 1. Changes of peel color (a*/b* ratio) (A) and juice content (B) of ‘Valencia’ orange fruit harvest from February to May 2012.
3.2 Peel oil and PME activity and pectin
Peel oil remained steady over the season with the exception of an
increase in the month of April (Fig. 2A). PME is an enzyme that demethylates
pectin in cell walls and can destabilize the cloud in orange juice (VERSTEEG et
al., 1980; CAMERON et al., 1998; ACKERLEY et al., 2002; BALDWIN et al.,
2012). PME activity mildly fluctuated over the season (Fig. 2B) while
galacturonic acid held steady in the entire harvest season (Fig. 2C) (BAI et al.,
2009).
Figure 2. Changes of peel oil content (A), pectin methylesterase (PME) activity (B), and total pectin (galacturonic acid) content (C) in ‘Valencia’ orange juice extracted from fruit harvested from February to May 2012.
Galacturonic acid is the main component of pectin. This is in contrast to
Sinclair and Jolliffe (1958; 1961) and Rouse et al. (1962) who observed that in
50
maturing oranges, total pectin and water-soluble pectic substances decreased
in the peel and pulp, in both California and Florida ‘Valencia’ fruit.
3.3 Sugars and acids
SSC (°Brix) of the juice increased from 15.5% to 16.5% over the harvest
season (Fig. 3A). However, TA content decreased consistently from over 1.4%
to under 1.0% (Fig. 3B). Consequently, SSC/TA ratio increased from 11 in
February to just over 17 in May (Fig. 3C). All juices passed Florida juice
standard (RITENOUR et al., 2004). A high quality juice has a SSC/TA ratio
between 12.5 and 19.5 (MATTHEWS, 1994). In this study, early harvested high
acid fruit had a SSC/TA ratio of 11, out of the best quality range.
Figure 3. Changes of soluble solids content (SSC) (A), titrable acidity (TA) (B), and SSC/TA ratio (C) in ‘Valencia’ orange juice extracted from fruit harvested from February to May 2012.
Citric acid, the principal organic acid, decreased throughout the harvest
season (Fig. 4A), similar to our previous study (BAI et al., 2009); however, malic
acid (9% to 15% of total organic acids) slightly decreased in the first month and
then increased from March to May (Fig. 4B). In mature orange juice sacs, both
aconitase and citrate lyase activities were absent (ECHEVERRIA & VALICH,
1988). The regulation of citrate formation may be by decreasing synthesis of
oxaloacetate, the precursor of citrate, during maturation (BRUEMMER, 1989),
explaining the decrease in citric acid.
Total ascorbic acid content decreased consistently during harvest
season (Fig. 4C), which is in agreement with Harding et al. (1940) and Rygg
and Getty (1955) and our last study (BAI et al., 2009).
51
Figure 4. Changes of citric (A), malic (B), and ascorbic (C) acids in ‘Valencia’ orange juice extracted from fruit harvested from February to May 2012.
3.4 Secondary metabolites
Several classes of secondary metabolites were measured in the
‘Valencia’ orange juice between February and May 2012. These classes of
compounds consisted of: phenolic compounds, limonoids, and alkaloids. The
phenolic compounds included the flavonoid glycosides (FGs), polymethoxylated
flavones (PMFs) and hydroxycinnamic acids (HCAs). All five FGs, hesperidin-
4’-glucoside, hesperidin, 6,8-di-C-glucosyl apigenin, isosakuranetin rutinoside
and narirutin, showed gradual increases through May (Fig. 5A-E); PMFs
including heptamethoxyflavone, quercetagetin hexamethylether, nobelitin,
tetramethylscutellarein, sinesetin, and tangeretin, increased steadily (Fig. 6A-F);
Nine of HCAs were detected without further identification, and the contents
decreased steadily (data not shown).
Five out of six limonoids (all the limonoid glucosides) increased, including
obacunone glucoside, nomilin glucoside, nomilinic acid glucoside, and limonin
glucoside (Fig. 7A-D). Of the two aglycones measured, limonin increased (Fig.
7E), while nomilin levels were steady (Fig. 7F). Feruloyl putrescine and an
unknown alkaloid increased after April (data not shown).
52
Figure 5. Changes of flavonoid glycosides (FGs, relative peak área) in ‘Valencia’ Orange juice extracted from fruit harvested from February to May 2012. (A) Hesperedin-4’-glucoside; (B) hesperidin; (C) 6,8-di-C-glucosyl apigenin; (D)
isosakuranetin rutinoside; (E) narirutin.
Figure 6. Changes of polymethoxylated flavones (PMFs, relative peak área) in ‘Valencia’ Orange juice extracted from fruit harvested from February to May 2012. (A) heptamethoxyflavone; (B) quercetagetin hexamethylether; (C) nobiletin; (D)
tetramethylscutellarein; (E) sinesetin; and (F) tangeretin.
53
Figure 7. Changes of limonoids (relative peak área) in ‘Valencia’ orange juice extracted from fruit harvested from February to May 2012. (A) Obacunone
glucoside; (B) nomilin glucoside; (C) nomilinic acid glucoside; (D) limonin glucoside; (E) limonin; and (F) nomilin.
3.5 Bioactive amines
Among 10 amines (putrescine, agmatine, spermine, spermidine,
cadaverine, serotonin, histidine, tyramine, tryptamine, phenylethylamine)
investigated, the polyamines spermidine, spermine, and putrescine were
detected in the samples. Putrescine was the prevalent amine, followed by
spermidine and spermine (Fig. 8).
Figure 8. Changes of (A) putrescine, (B) spermidine, and (C) spermine in ‘Valencia’ orange juice extracted from fruit harvested from February to May 2012.
54
No changes were observed for putrescine; however, there was an
increase in spermidine and spermine levels with harvest time (Fig. 8B). An
increase in spermidine levels during ripening was reported by Tassoni et al.
(2004) for Brasiliano NL92 orange, followed by a decrease in over ripened
oranges.
3.6 Volatiles
Instead of direct headspace method used in the last study, this research
used SPME extraction, and thus detected more volatile compounds. In the total
97 compounds, there were 18 monoterpene hydrocarbons, 22 sesquiterpene
hydrocarbons, 9 aliphatic esters, 4 terpene esters, 12 aliphatic aldehydes, 3
terpene aldehydes, 4 aliphatic alcohols, 5 terpene alcohols, 4 ketones and 1
acid, with the rest being minor or unidentified components (Table 1).
Limonene was the major component, representing 85% of total volatiles,
throughout the entire harvest season. The concentration decreased in April and
recovered in May. Most of groups and chemicals had higher concentrations in
April and/or May than earlier in the season, agreeing with the results observed
in the last study (BAI et al., 2009). However, both aliphatic and terpene alcohols
did not have differences between harvest time as a group
55
Table 1. Effect of harvest time on volatile abundance in ‘Valencia’ orange juice (2012)z
Compound Volatile abundance (total ion current x 107)
RIY AOX Feb Mar Apr May
Monoterpene hydrocarbons
limonene 1046 1 1411 ab 1382 ab 1113 b 1649 a
β-myrcene 997 5 15.04 b 12.68 b 26.39 a 21.18 ab
α-pinene 953 8 8.92 7.47 5.86 10.52
α-terpinene 1031 14 3.32 2.94 3.34 4.57
γ-terpinene 1069 15 1.59 b 1.61 b 5.54 a 4.28 a
α-phellandrene 1022 18 3.79 1.03 1.26 4.17
β-phellandrene 1048 22 0.00 c 0.00 c 5.40 a 2.13 b
p-cymene 1039 30 1.61 1.51 0.83 0.62
δ-3-carene 1020 34 0.94 ab 0.77 bc 1.02 a 0.59 c
α-thujene 942 39 0.82 0.76 0.49 0.81
mtw1197 1197 44 0.37 b 0.34 b 0.33 b 0.94 a
isolimonene 1081 49 0.37 0.36 0.44 0.51
sabinene 990 59 0.31 b 0.28b 0.34 ab 0.41 a
1,3,8-p-menthatriene- 1041 67 0.36 0.17 0.15 0.16
p-mentha-6,8-dien-2-ol 1146 74 0.00b 0.00b 0.60 a 0.00 b
p-mentha-2,4(8)-diene 1098 75 0.24 0.09 0.19 0.07
β-ocimene 1238 80 0.00 b 0.09 b 0.10 b 0.31 a
mt1332 1348 91 0.08 0.00 0.00 0.11
total (excluding limonene) 37.78 b 30.10 b 52.28 a 51.38 a
Sesquiterpene hydrocarbons
valencene 1536 2 86.50 b 78.65 b 142.81 a 114.83 ab
stw1526 1526 6 11.50 b 10.28 b 21.44 a 11.63 b
st1526 1574 12 4.55 5.41 1.58 4.82
α-selinene 1542 13 1.71 b 1.17 b 10.53 a 1.96 b
α-cadinene 1554 16 2.09 b 3.01 ab 3.30 ab 3.80 a
st1454 1454 17 2.40 2.13 3.63 3.42
st1405 1405 21 1.19 b 1.40 b 2.60 a 2.56 a
α-copaene 1397 23 3.71 0.48 3.30 0.00
st1548 1548 24 0.84 b 1.24 b 3.38 a 1.13 b
cedrane-V6 1518 26 1.27 b 4.42 a 0.25 ab 0.19 b
α-caryophllene 1479 28 0.00 0.00 3.66 1.83
α-farnesene 1507 29 1.07 b 1.01 b 1.05 b 1.50 a
β-panasinsen 1563 37 0.79 0.81 0.87 0.050
β-cubebene 1358 51 0.46 0.42 0.50 0.23
56
Table 1. Effect of harvest time on volatile abundance in ‘Valencia’ orange juice
(2012)z (continuation…)
Compound Volatile abundance (total ion current x 107)
RIY AOX Feb Mar Apr May
Sesquiterpene hydrocarbons
β-selinene 1740 55 0.37 0.35 0.35 0.40
β-curcumene 1532 60 0.24 0.23 0.47 0.40
st1500 1500 63 0.89 0.00 0.41 0.00
st1348 1332 81 0.14 0.12 0.13 0.10
st1577 1577 85 0.07 0.04 0.09 0.12
β-pamasinsene 1513 86 0.00 0.00 0.18 0.11
alloaromadendrene 1462 88 0.00 0.00 0.03 0.18
β-humulene 1475 92 0.00 b 0.00 b 0.18 a 0.00
total 119.80 b 111.17 b 200.73 a 149.73 ab
Aliphatic esters
ethyl butanoate 801 3 31.72 b 37.81 b 41.36 ab 49.92 a
ethyl pentanoate 883 9 6.12 b 5.63 ab 5.78 ab 8.35 a
ethyl 3-hydroxyhexanoate 1124 19 1.87 ab 2.22 b 2.31 ab 2.85 a
ethyl acetate 600 31 0.89 b 1.03 ab 1.12 ab 1.39 a
ethyl 2-methylbutanoate 854 40 0.00 b 0.49 b 2.36 a 0.00 b
ethyl octanoate 1184 42 1.09 b 0.00 ab 1.03 ab 0.00 a
methyl hexanoate 929 54 0.25 0.30 0.35 0.59
methyl butanoate 715 57 0.31 0.32 0.41 0.31
Z-5-dodecen-1-y1 acetate 1596 62 0.31 0.41 0.22 0.37
total 42.56 b 48.23 b 54.92 ab 63.78 a
Terpene esters
neryl acetate 1347 25 0.93 b 0.99 b 2.42 a 2.24 a
citronellyl acetate 1337 35 0.61 b 0.59 b 0.66 b 1.24 a
terpinyl acetate 1202 47 0.65 0.31 0.37 0.39
carvyl acetate 1328 76 0.00 c 0.17 b 0.03 c 0.34 a
Total 2.19 bc 2.07 c 3.47 ab 4.21 a
Aliphatic aldehydes
Z-3-hexenal 863 7 7.26 9.02 14.68 12.47
hexanal 804 11 2.33 0.49 8.48 5.54
E,E-2,4-decadienal 1270 20 1.50 b 1.67 ab 2.17 ab 2.52 a
octanal 1010 38 0.00 b 0.60 b 0.60 1.71 a
decanal 1200 41 0.52 0.57 0.53 0.60
nonanal 1104 45 0.23 b 0.30 b 0.83 a 0.61 ab
acetaldehyde 466 53 0.00 b 0.24 ab 1.06 a 0.29 ab
57
Table 1. Effect of harvest time on volatile abundance in ‘Valencia’ orange juice
(2012)z (continuation…)
Compound Volatile abundance (total ion current x 107)
RIY AOX Feb Mar Apr May
Aliphatic aldehydes
heptanal 911 68 0.34 0.16 0.13 0.16
E-2-octenal 1062 78 0.35 a 0.21 ab 0.20 ab 0.00 b
E-2-heptenal 968 84 0.19 0.08 0.15 0.09
pentenal 672 93 0.00 b 0.00 b 0.33 a 0.00 b
Z-dodec-5-enal 1378 0.04 0.03 0.10 0.00
total 12.76 b 13.38 b 29.26 a 24.00 a
Terpene aldehydes
perilla aldehyde 1288 43 0.27 b 033 b 0.61 a 0.79 a
geranial 1263 73 0.12 0.10 0.21 0.20
neral 1236 90 0.12 a 0.00 b 0.03 ab 0.04 ab
total 0.52 bc 0.43 c 0.85 ab 1.03 a
Aliphatic alcohols
ethanol 487 4 17.87 17.87 17.83 22.50
undecanol 1364 56 0.05 0.20 1.14 0.00
hexanol 873 66 0.28 0.23 0.11 0.29
2-methyl-decanol 1322 70 0.00 0.18 0.14 0.40
total 18.19 18.48 19.21 23.19
Terpene alcohols
linalool 1100 10 5.69 6.08 4.45 3.93
terpinen-4-ol 1191 32 0.78 b 0.75 b 1.07 ab 1.51 a
E-carveol 1413 33 0.49 0.52 1.39 1.14
citronellol 1217 65 0.12 b 0.18 ab 0.54 a 0.26 ab
nerol 1220 95 0.00 0.00 0.00 0.12
total 7.07 7.53 7.46 6.97
Ketones
2-pentanone 676 27 1.30 1.22 1.93 1.15
β-ionone 1426 46 0.63 a 0.47 ab 0.46 ab 0.29 b
geranylacetone 1436 83 0.08 0.12 0.11 0.03
nootkatone 1892 50 0.00 b 0.00 b 1.63 a 0.00 b
total 2.01 b 1.81 b 4.13 a 1.47 b
Other
hexanoic acid 965 72 0.00 0.00 0.33 0.33
riw923 923 36 0.55 0.45 0.96 1.07
benzene 1496 48 0.30 0.41 0.67 0.32
58
Table 1. Effect of harvest time on volatile abundance in ‘Valencia’ orange juice
(2012)z (continuation…)
Compound Volatile abundance (total ion current x 107)
RIY AOX Feb Mar Apr May
Other
ri1071 1071 52 0.27 0.24 0.52 0.58
ri1743 1743 58 0.22 c 0.27 bc 0.50 a 0.35 b
ri1251 1251 61 0.37 0.34 0.16 0.46
tetradecane 1389 64 0.34 0.21 0.36 0.30
ri1317 1317 71 0.38 0.13 0.17 0.00
ri1300 1300 77 0.14 0.12 0.19 0.08
ri1936 1936 79 0.00 b 0.00 b 0.19 a 0.33 a
ri1711 1711 82 0.00 b 0.00 b 0.23 a 0.00 b
ri1391 1391 87 0.00 b 0.00 b 0.23 a 0.00 b
ri1732 1732 89 0.00 0.00 0.13 0.08
ri1724 1724 94 0.00 b 0.00 b 0.16 a 0.00 b
ri1619 1619 96 0.00 b 0.00 b 0.11 a 0.00 b
ri1697 1697 97 0.00 b 0.00 b 0.09 a 0.00 b
total 2.57 b 2.23 b 5.05 a 3.89 b
total (excluding limonene) 202 b 192 b 311 a 269 a
ZValues followed by different letters in the same compound (row) are significantly different at P=0.05 using Tukey`s test. yRI: retention index. xAO: abundance order from compound with the highest amount. wnonidentified monoterpene (mt), sesquiterpene (st) and other compounds (ri) followed by the RI values.
4. CONCLUSION
‘Valencia’ oranges are harvested generally from March to June. Because
of unusually warm weather, the 2012 harvest season was started in February
and ended in May (rather than normally March to June). The mid season
harvests are preferred for the optimum SSC, TA, SST/TA, reduced bitterness.
Later-harvested ‘Valencia’ fruit had higher color, soluble solids, solid/acid ratio,
volatiles, flavonoids, spermidine and limonoid glycoside contents while having
reduced juice content, acids (including ascorbic acid) and limonin and nomilin
(in May).
59
CAPÍTULO II - EFFECT OF HUANGLONGBING (GREENING
DISEASE) ON ORANGE JUICE QUALITY, A REVIEW
ABSTRACT
Huanglongbing (HLB) or citrus greening is one of the most severe citrus
diseases in the world. It is associated with the presence of the gram-negative
bacterium Candidatus Liberibacter asiaticus which is transmitted by the psyllid
Diaphorina citri Kuwayama (Hemiptera: Psyllidae) and also the African species,
Candidatus Liberibacter africanus, which is transmitted by the insect Trioza
erytreae (Hemiptera: Triozidae). Fruits from a tree infected with HLB’s bacteria
can be either symptomatic or asymptomatic. Symptomatic fruits are small in
size, lopsided, and asymmetrical with a green peel. The disease has a negative
impact on fruit quality and results in off-flavored orange juice. Symptomatic
fruits show higher total acidity (TA) and lower soluble solids content (SSC),
SSC/TA, total sugar content and malic acid levels compared to healthy and
asymptomatic fruit. The disease also causes an increase in secondary
metabolites, including: hydroxycinnamic acids; bitter limonoids (limonin and
nomilin), narirutin and hesperidin in the orange juice, peel and pulp. Typical
HLB orange juice is described as being distinctly bitter, sour, salty/umami,
metallic, pungent, musty, and lacking in sweetness and citrusy flavor. However,
the changes in volatile compounds have not been well established, except for
the increase in numerous limonene and linalool degradation compounds, as
well as a decrease in some aldehydes. The most studied orange cultivar is
Valencia, followed by Hamlin. HLB remains without a cure and its management
is difficult due to an unpredictable latency time of the bacteria after the tree has
been infected. The scientific literature is still lacking scientific information
covering the effects of HLB on orange juice quality, as well as investigations on
cultivars other than Valencia and Hamlin.
KEYWORDS: Huanglongbing. Candidatus Liberibacter asiaticus. Orange juice.
Valencia. Hamlin. Quality.
Artigo submetido a publicação no Journal of the Science of Food and
Agriculture.
DALA PAULA, B.M.; FERRAREZI, R.S.; PLOTTO, A.; GLÓRIA, M.B.A.
60
1. INTRODCUTION
Huanglongbing (HLB) is a citrus disease that may bring an end to the
citrus industry if the disease continues to spread throughout the various citrus
growing regions of the world (GOTTWALD et al., 2012). Practically all
commercial citrus species and cultivars are vulnerable to HLB. The disease has
an array of symptoms which can be present anywhere from the roots to the
citrus fruit itself, changing the chemical characteristics and sensory attributes of
the fruits (BOVÉ, 2006; BALDWIN et al., 2010; DALA PAULA et al., 2017a;
2017b). In this review, the effects of HLB on orange juice quality is described
based on research available in the scientific literature.
2. WORLDWIDE CONSUMPTION AND PRODUCTION OF FRESH ORANGES
AND ORANGE JUICE
Orange juice is the most widely consumed fruit juice in the world, with a
consumption of 7,574 out of 16,988 million L in 2015, representing 45% of total
fruit juice consumption (MARKSTRAT, 2016). Brazil is the world's largest
orange producer, and reached production levels of approximately 14,350 metric
tons in the harvest of 2015/2016. China is the second largest producer with
7,000, followed by the European Union – 6,055, the United States – 5,371 and
Mexico – 3,535 metric tons (USDA-FAS, 2017). In the 2015-2016 harvest,
Brazilian and American commercial orange production occupied approximately
741,133 and 223,143 hectares, respectively (IBGE-SIDRA, 2017, USDA-NASS,
2017). While the majority of the orange production in Brazil is processed and
exported, the U.S. consumes practically all of its production and imports juice
from other countries, including Brazil, in order to meet its market demand.
Florida accounts for nearly 60% of U.S. production, with California accounting
for the remaining 40%. Around 90% of the oranges produced in Florida are
processed (USDA-FAS, 2017).
Currently, citrus producers in many countries are facing serious problems
with the emergence of the plant pathology HLB (TEIXEIRA et al., 2008;
BASSANEZI et al., 2009; 2011; SPREEN & ZANSLER, 2015), which means
61
yellow dragon disease in Chinese and is also known as citrus greening
(HALBERT & MANJUNATH, 2004). HLB is considered one of the most severe
citrus diseases in the world and, consequently, a serious problem for the citrus
processing industry. The disease can affect almost all kinds of citrus, with sweet
oranges, tangelos and mandarins being the most susceptible and limes, sour
oranges and trifoliate oranges being the least (ABDULLAH et al., 2009).
3. A BRIEF HISTORICAL BACKGROUND OF HUANGLONGBING
INCIDENTS
It is difficult to determine where exactly the HLB disease originated.
However, there is evidence suggesting that HLB was responsible for India’s
“dieback” problem during the 18th century and for Yellow shoot in China in the
1890s (CAPOOR, 1963; ZHAO, 1981; GRAÇA, 2008). Initially, some
researchers believed that the tristeza virus was the leading cause for the citrus
“dieback” in India, however contradictory evidence supported other arguments.
For example, many of the affected species that died in India are tolerant of
tristeza when they are grown in other countries. After a three-month survey
conducted in India by Fraser et al. (1966), HLB was determined to be the
primary cause of the “dieback” (FRASER & SINGH, 1968; GRAÇA, 2008). In
1937, the disease was described for the first time in South Africa (VAN DER
MERWE et al., 1937), and it was later linked to chromium and manganese
toxicity. It was also associated with the leaf mottling citrus disease in the
Philippines in the 1960’s (FRASER et al., 1966; MCCLEAN & SCHWARZ,
1970). Currently, the disease has spread out to more than 50 countries (Figure
1) in Africa, Asia, Oceania and the Americas (South, North, Central American
and the Caribbean) (CABI, 2017; EPPO, 2017).
The first case of this century-old disease in America was reported in the
state of São Paulo (SP), Brazil in 2004 (COLLETTA-FILHO et al., 2004;
TEIXEIRA et al., 2005a). However, in a survey conducted in SP, just six months
after HLB had been reported in Brazil, 46 cities stated having infected trees,
suggesting that HLB had been present for almost ten years (Bové 2006). A year
later, in August 2005, symptoms of the disease were recognized in Florida,
U.S.; in 2007 in Cuba; in 2008 in the Dominican Republic; and in 2010 in
62
Mexico (COLLETA-FILHO et al., 2004; HALBERT, 2005; LLAUGER et al.,
2008; MATOS et al., 2009; NAPPO, 2010). Currently, HLB is present in all
Florida citrus-growing counties (BALDWIN et al., 2010), in California, Georgia,
Louisiana, South Carolina and Texas (CABI, 2017; EPPO, 2017). As the
severity of HLB increases, premature fruit drop becomes a growing problem,
which has contributed to declining yields in Florida, especially during the last
few years (CHEN et al., 2016). In Brazil, SP, Minas Gerais and Paraná have
reported the presence of HLB, with SP being the most affected state. In India
and China, HLB has spread to around 25 and 11 states, respectively (Table 1)
(CABI, 2017; EPPO, 2017).
Figure 1. Countries currently affected by Huanglongbing – HLB. (CABI, 2017;
EPPO, 2017).
63
Table 1. Worldwide distribution of Huanglongbing’s bacteria and vectors.
Country Bacteria Status Vector Status
Asia
Afghanistan - - Diaphorina citri present
Bangladesh CLas present Diaphorina citri present
Bhutan CLas present Diaphorina citri present
Cambodia CLas present Diaphorina citri present
China CLas present (Fujian, Guangdong, Guangxi, Guizhou, Hainan, Hunan, Jiangxi, Schuan, Yunnan, Zhejiang); few occurrences (Xianggang - Hong Kong)
Diaphorina citri present (Aomen, Fujian, Guangdong, Guizhou, Hainan, Henan, Hunan, Jiangxi, Sichuan, Yunnan, Zhejiang); widespread (Xianggang); restricted distribution (Guangxi)
East Timor CLas widespread Diaphorina citri present
India CLas present (Andhra Pradesh, Arunachal Pradesh, Assam, Bihar, Delhi, Gujarat, Haryana, Himachal Pradesh, Jammu & Kashmir, Karnataka, Kerala, Madhya Pradesh, Maharashtra, Manipur, Meghalaya, Mizoram, Nagaland, Orissa, Punjab, Rajasthan, Sikkim, Tamil Nadu, Tripura, Uttar Pradesh, West Bengal)
Diaphorina citri present (Andhra Pradesh, Arunachal Pradesh, Assam, Bihar, Delhi, Gujarat, Haryana, Himachal Pradesh, Jammu & Kashmir, Karnataka, Kerala, Lakshadweep, Madhya Pradesh, Maharashtra, Manipur, Meghalaya, Punjab, Rajasthan, Sikkim, Tamil Nadu, Tripura, Uttar Pradesh, West Bengal)
Indonesia CLas present (Irian Jaya, Java, Kalimantan, Sulawesi, Sumatra); widespread (Nusa Tenggara)
Diaphorina citri present (Java, Maluku, Nusa Tenggara, Sumatra);
Iran CLas restricted distribution Diaphorina citri restricted distribution
Japan CLas present (Ryukyu Archipelago); restricted distribution (Kyushu)
Diaphorina citri present, few occurrences (Kyushu); present (Ryukyu Archipelago)
Laos CLas present Diaphorina citri present
Malaysia CLas present (Sarawak, West) Diaphorina citri present (Sabah, West)
Maldives - - Diaphorina citri present
Myanmar CLas present Diaphorina citri present
Nepal CLas widespread Diaphorina citri present
Oman - - Diaphorina citri restricted distribution
Pakistan CLas present Diaphorina citri widespread
Philippines CLas widespread Diaphorina citri present
Saudi Arabia CLaf present Trioza erytreae Diaphorina citri
restricted distribution present
Sri Lanka CLas present Diaphorina citri present
Taiwan CLas present widespread Diaphorina citri restricted distribution
Thailand CLas present Diaphorina citri present
64
Country Bacteria Status Vector Status
United Arab Emirates - - Diaphorina citri present
Vietnam CLas present restricted distribution Diaphorina citri restricted distribution
Yemen CLaf present restricted distribution Trioza erytreae Diaphorina citri
restricted distribution present
Africa
Angola - - Trioza erytreae present
Burundi CLaf present - -
Cameroon CLaf present Trioza erytreae present
Camoros - - Trioza erytreae present
Congo, Democratic republic of the
- - Trioza erytreae restricted distribution
Central African Republic CLaf present - -
Eritrea - - Trioza erytreae present
Ethiopia CLaf CLas
present present (few occurrences)
Trioza erytreae present
Kenya CLaf present Trioza erytreae present
Madagascar CLaf present Trioza erytreae present
Malawi CLaf present Trioza erytreae present
Mauritius CLaf CLas
present restricted distribution
Trioza erytreae Diaphorina citri
present present
Réunion CLaf CLas
present restricted distribution
Trioza erytreae Diaphorina citri
present present
Rwanda CLaf present Trioza erytreae present
Saint Helena CLaf present (widespread) Trioza erytreae present
Sao Tome & Principe - - Trioza erytreae present
Somalia CLaf present - -
South Africa CLaf restricted distribution Trioza erytreae widespread
Sudan - - Trioza erytreae present
Swaziland CLaf present Trioza erytreae restricted distribution
Tanzania CLaf restricted distribution Trioza erytreae Diaphorina citri
restricted distribution restricted distribution
Uganda - - Trioza erytreae present
Zambia - - Trioza erytreae present
Zimbabwe CLaf restricted distribution Trioza erytreae present
65
Country Bacteria Status Vector Status
North America
Mexico CLas restricted distribution Diaphorina citri restricted distribution
USA CLas present, few occurrences (California, Georgia, Louisiana, South Carolina, Texas); widespread (Florida)
Diaphorina citri present (Florida, Hawai, Texas); few occurrences (Alabama, California, Georgia, Louisiana, Mississippi, South Carolina); restricted distribution (Arizona)
Central America
Antigua and Barbuda - - Diaphorina citri present
Bahamas - - Diaphorina citri present
Barbados CLas restricted distribution Diaphorina citri restricted distribution
Belize CLas restricted distribution Diaphorina citri present
Cayman Islands - - Diaphorina citri present
Costa Rica CLas restricted distribution Diaphorina citri present
Cuba CLas present (widespread) Diaphorina citri present
Dominica CLas
restricted distribution Diaphorina citri present
Dominican Republic CLas
restricted distribution Diaphorina citri present
Guadeloupe CLas
restricted distribution Diaphorina citri restricted distribution
Haiti - - Diaphorina citri present
Honduras CLas
present (few occurrences) - -
Jamaica CLas
present (widespread) Diaphorina citri present
Martinique CLas
restricted distribution Diaphorina citri present
Nicaragua CLas
present - -
Puerto Rico CLas
present Diaphorina citri present
United States Virgin Islands
CLas present (few occurrences) Diaphorina citri present
66
Country Bacteria Status Vector Status
South America
Brazil CLas CLam
present (Minas Gerais, Paraná, São Paulo) present (Minas Gerais, Paraná, São Paulo)
Diaphorina citri present (Amazonas, Bahia, Ceará, Minas Gerais, Pará, Paraná, Pernambuco, Rio de Janeiro, Santa Catarina, São Paulo)
Columbia CLas
present (few occurrences) Diaphorina citri widespread
Paraguay CLas. restricted distribution Diaphorina citri restricted distribution
Uruguay - - Diaphorina citri few occurrences
Venezuela - - Diaphorina citri restricted distribution
Europe
Portugal - - Trioza erytreae restricted distribution
Spain - - Trioza erytreae restricted distribution
Oceania
American Samoa - - Diaphorina citri present
Guam - - Diaphorina citri present
Papua New Guinea CLas restricted distribution Diaphorina citri restricted distribution
Leg.: CLas: Candidatus Liberibacter asiaticus; CLaf: Candidatus Liberibacter africanus; CLam: Candidatus Liberibacter americanus.
67
4. CAUSING AGENTS AND VECTORS OF HUANGLONGBING
It is well established that HLB is associated with the presence of the gram-
negative bacteria genus Candidatus Liberibacter (CL). Three species are known
to cause the symptoms of HLB – CL asiaticus (CLas), CL americanus (CLam)
and CL africanus (CLaf). The Asian and the recently discovered American
species, in Brazil, can be transmitted by the psyllid Diaphorina citri Kuwayama
(Hemiptera: Psyllidae) and the African species by the insect Trioza erytreae
(Hemiptera: Triozidae) (Figure 2) (BOVÉ, 2006). Although HLB was first
reported in Brazil and the US 15 years ago, the psyllid vector was reported in
SP and Florida as early as 1942 and 1998, respectively (BOVÉ, 2006; TANSEY
et al., 2017).
Figure 2. Development stages of Diaphorina citri Kuwayama (Hemiptera: Psyllidae) (upper) and Trioza etrytreae (Del Guercio) (Hemiptera: Triozidae) (lower). (Cheraghian, 2013).
When the symptoms of HLB in orange trees were reported for the first
time in Brazil, symptomatic and asymptomatic leaves from sweet orange trees
were analyzed for the presence of CLas and CLaf by polymerase chain reaction
(PCR) using two sets of HLB-specific primers for amplification of 16S rDNA and
ribosomal protein genes. All samples tested using PCR amplification were
68
negative, however HLB-affected leaves from the Bordeaux HLB collection were
positive. Thus, researchers analyzed the samples again using PCR with
universal primers for amplification of bacterial 16S rDNA and found that all
symptomatic leaves yielded the same 16S rDNA amplification product.
Afterwards, to confirm the existence of bacteria in symptomatic leaves, the 16S
rDNA product was cloned, sequenced and compared with those of CLas and
CLaf. The homology between the sequences was 93.7% and 93.9%,
respectively, while the homology of the two known Liberibacter species was a
97.5% sequence identity. Thus, the bacterium was classified as a new species
(TEIXEIRA et al., 2005b).
CLam was the most prevalent bacteria species in Brazil in 2005, which
initially affected more than 90% of the infected trees, decreasing to 60% in
2007. During this period, there was an increase in CLas infection, from 5 to 35%
of the infected trees, while a combined infection remained practically the same
at 5% (COLETTA-FILHO et al., 2007; GASPAROTO et al., 2012). Among HLB’s
bacteria, CLaf is sensitive to heat and to dry weather and thrives between 20
and 25 ºC, while the other species are heat tolerant and thrive just as well at
higher temperatures (CATLING, 1969; CHERAGHIAN, 2013).
5. Symptoms of Huanglongbing and its impact on orange trees
It is uncertain how long a tree can be infected before showing the
symptoms of the disease but, when it eventually becomes symptomatic,
symptoms manifest on different parts of the tree. Infected trees generally have
open growth, stunting, twig dieback and discolored leaves, which appear in
contrast to the other healthy or symptomless parts of the tree. The symptomatic
leaves can be normal-sized, showing yellow coloration and development of a
blotchy-mottle or they can be small, upright and show a variety of chlorotic
patterns resembling those induced by zinc or other nutritional deficiencies
(Figure 3) (MCCLEAN & SCHWARZ, 1970; GRAÇA, 1991; ALBRECHT et al.,
2016). The root systems are poorly developed, showing very few fibrous roots,
which decay from the rootlets most likely due to starvation (GRAÇA, 1991;
BATOOL et al., 2007).
69
Figure 3. HLB symptomatic orange leaves: symptomatic normal sized leaves
with development of blotchy-mottle (on left) (BOVÉ, 2006); and symptomatic
small sized leaves (on right) (EMBRAPA, 2011).
Along with the color changes in the leaves, there are some changes in
metabolic composition. HLB affects the profile of hydroxycinnamic acids and
flavonoids in infected leaves, resulting in lower levels of 6,8-di-C-glucosyl
apigenin, apigenin-C-glucosyl-O-xyloside, 2”-xylosylvitexin, luteolin rutinoside
and apigenin-7-O-rutinoside compared to healthy leaves. While healthy leaves
contain only trace levels of limonin glucoside, infected leaves contain levels of
300 ± 22 µg/mL (MANTHEY, 2008). Metabolomic analysis using gas
chromatography-mass spectrometry (GC-MS) of Valencia sweet orange leaves
has been suggested to identify biomarkers for rapid differentiation of HLB
infection from zinc deficiency. The combination of L-proline, β-elemene, (-)trans-
caryophyllene and α-humulene as HLB biomarkers, is necessary to increase
specificity, because the change in concentration of a single compound may not
be exclusively attributed to HLB (Cevallos-Cevallos et al., 2011). Tolerance of
HLB does not seem to be linked to the accumulation of higher levels of
protective metabolites in response to infection, but rather to different
concentrations of specific metabolites independent of infection (ALBRECHT et
al., 2016).
With respect to the orange fruit, they are reduced in size, lopsided,
asymmetric, and contain small, brownish/black aborted seeds which can be
seen when the orange is sectioned perpendicularly to the fruit axis (Figure 4).
The orange peel turns green with an inversion of colors—when the fruit starts to
70
change color, from green to yellow/orange, the peduncular end turns orange
while the stylar end remains green. In a healthy orange, CLas (-), the color
change first starts at the stylar end, progressing only later to the peduncular
area (Figure 4). HLB causes fruits to drop prematurely, resulting in a 30-100%
yield reduction, and, ultimately, premature death of the tree. Tree mortality can
occur several months to years after infection (MCCLEAN & SCHWARZ, 1970;
GRAÇA, 1991; BOVÉ, 2006; BATOOL et al., 2007; BASSANEZI et al., 2011;
LIAO & BURNS, 2012).
Figure 4. Typical HLB symptomatic orange: (upper right and upper left)
asymmetric fruit containing small, brownish aborted seeds (EMBRAPA, 2011;
INIAV, 2015); (lower left) normal change of color in a healthy orange, CLas (-)
(EMBRAPA, 2011); and (lower right) inversion of colors in a typical HLB
symptomatic orange, CLas (+) (INIAV, 2015).
Research found in the scientific literature shows that HLB symptomatic
fruits from infected trees are smaller in diameter compared to asymptomatic and
healthy fruits, which are shown to have similar diameters (Table 2 and Figure
5). The majority of the research also reports that the weights and juice contents
of symptomatic oranges are diminished compared to asymptomatic and healthy
oranges, which are reported to generally be similar in weight and juice content
(Table 2 and Figure 5). Most of the published research analyzed Valencia and
Hamlin oranges, and in one study similar tendencies were described in the
Valencia Americana, Westin and Pera Rio cultivars. The differences caused by
71
the disease were the least notable in Valencia Americana cultivar, while the
most significant differences were observed in Valencia oranges, followed by
Westin oranges (BASSANEZI et al., 2009).
Table 2. Effects on diameter, weight and juice content in fruit affected by
Huanglongbing.
AS: asymptomatic; SY: symptomatic; 1Blend of oranges harvested on Sep. 2004, Jul. and Oct. 2005 and Aug. 2007; 2Blend of oranges harvested on Mar. and May 2013; 3Blend of oranges harvested on Jul. 2007, Jun. and Jul. 2008.
Values from the same reference with the same letter within columns are not significantly by the
following statistical analysis (It test with the probability of error estimated to be lower than
0.000); IIDuncan’s multiple range test P<0.01; IIITukey test at P ≤ 0.05).
HLB potentially causes trees to be more susceptible to other pest
concerns including citrus longhorned beetle (Anoplophora chinensis Forster)
attacks. In advanced cases of HLB infection, a combination of citrus longhorned
beetles and Phytophthora fungi is common (HALBERT & MANJUNATH, 2004;
BATOOL et al., 2007).
Reference Orange sample Fruit parameters
harvest time status or conditions
diameter (mm)
weight (g) juice (g.100 g-1)
Valencia orange juice
Bassanezi et al. (2009)I
Blend of different harvests1
HLB-AS
HLB-SY
73.1a
59.2b
208.1a
118.9b
50.0a
44.6b
Liao and Burns (2012)II
April 2009 Healthy
HLB-AS
HLB-SY
73.7a
76.5a
58.4b
208.5a
214.5a
122.3b
53.2a
52.9a
46.1b
Massenti et al. (2016)III
March and May 20132
Healthy
HLB-AS
HLB-SY
- 183b
208a
115c
58.9a
57.8ab
55.5b
Hamlin orange juice
Bassanezi et al. (2009)I
Blend of different harvests3
HLB-AS
HLB-SY
69.1a
60.5b
173.1a
128.6b
42.2a
39.3b
Liao and Burns (2012)II
December 2007 Healthy
HLB-AS
HLB-SY
71.5a
68.8a
53.2b
194.3a
196.6a
109.9b
52.1a
49.9a
48.8a
72
Figure 5. Symptomatic (left) and asymptomatic orange (middle) of HLB disease,
CLas (+); and healthy oranges (right), CLas (-) (SLIZS et al., 2012).
6. Fresh oranges and orange juice quality affected by Candidatus
Liberibacter asiaticus
To better understand the influence of HLB on the chemical and
physicochemical characteristics of orange juice, it is important to consider the
factors which may affect them, such as, cultivar, harvest date, location, degree
of maturity and the presence of pulp in the juice. In general, variation due to
harvest date is more dramatic compared to variation due to the disease
(BASSANEZI et al., 2009; BALDWIN et al., 2010; PLOTTO et al., 2010; BAI et
al., 2013; RAITHORE et al., 2015). As the season progresses, the peel color of
a healthy orange becomes less green and more orange, juice content declines,
sugars and SSC increase and TA, citric acid and total ascorbic acid levels tend
to decline (BAI et al., 2013).
6.1 Effects on physicochemical and biochemical characteristics
6.1.1 Peel color
As peel color often determines the attractiveness of an orange to the
consumer, the effects of HLB on this important characteristic are of great
concern within the citrus industry. Symptomatic oranges, CLas (+), are greener
or less orange in peel color compared to asymptomatic and healthy oranges.
Three studies have covered changes in peel color due to infection. Two of them
analyzed Hamlin oranges and reported a less orange colored peel in
73
symptomatic fruits. All three analyzed Valencia oranges, however only two
reported symptomatic fruits having less orange color in their peels, suggesting
that the Valencia orange cultivar seems to be the least affected by HLB,
regarding changes in peel color (BALDWIN et al., 2010; LIAO & BURNS, 2012;
MASSENTI et al., 2016).
6.1.2 Physicochemical characteristics
The physicochemical characteristics of oranges play a vital role in
determining the quality of the orange juice produced. There is no general
agreement among available results in the scientific literature regarding pH due
to status of CLas infection. The pH results of asymptomatic orange juice were
either higher, lower, or similar compared to healthy orange juice (PLOTTO et
al., 2008; PLOTTO et al., 2010; RAITHORE et al., 2015; DALA PAULA et al.,
2017b).
TA, SSC and SSC/TA tend to be similar in asymptomatic, CLas (+), and
healthy orange juice. However, a few studies reported differences in SSC/TA
between asymptomatic and healthy Valencia and Hamlin orange juices
(BALDWIN et al., 2010; DAGULO et al., 2010; MASSENTI et al., 2016). HLB
symptomatic juice usually presents the highest TA, and the lowest SSC and
SSC/TA in Valencia, Hamlin (Tables 3 and 4), Westin and Pera Rio orange
juices (BASSANEZI et al., 2009). SSC/TA, a parameter commonly used as a
fruit maturity index, tends to increase at later harvest dates and is more heavily
influenced by harvest time and orange cultivar than HLB infection status
(BALDWIN et al., 2010). Among the orange cultivars investigated, evaluation of
the effects of HLB predominantly addresses Valencia oranges.
74
Table 3. Physicochemical characteristics of Valencia orange juice made with
healthy fruit and fruit at different stages of HLB infection.
Reference
Orange juice sample Physicochemical characteristics
harvest time status or conditions
pH TA (g.100 mL-1)
SSC (°Brix)
SSC/TA
Valencia orange juice
Plotto et al. (2008)I
July 2006
Healthy FJ HLB FJ Healthy JWP HLB JWP
4.62b 4.78a 4.60b 4.74b
0.64a 0.54b 0.63a 0.47c
12.0a 11.3a 11.6a 10.1b
18.8b 21.0b 18.3b 21.6a
Bassanezi et al. (2009)II
Blend of different harvests1
HLB-AS HLB-SY
- 1.22a 1.75b
9.6a 8.0b
8.3a 4.8b
Baldwin et al. (2010)I
March 2007 April 2007 May 2007 June 2007
Healthy HLB-AS Healthy HLB-AS Healthy HLB-AS Healthy HLB-AS
-
0.82Aa 0.84Aa 0.68Ba 0.72Ba 0.57Ca 0.54Ca 0.43Da 0.41Da
10.7ABa 10.3Aa 10.1Ba 9.7Aa
10.6Ba 9.6Ab
11.0Aa 10.1Ab
13.2Da 12.5Da 15.1Ca 13.6Ca 18.6Ba 18.0Ba 25.8Aa 24.8Aa
Dagulo et al. (2010)III
April 04, 2008 April 18, 2008 May 23, 2008
Healthy HLB-AS HLB-SY Healthy HLB-AS HLB-SY Healthy HLB-AS HLB-SY
- - -
13.7a 10.8b 5.10c 14.8a 13.0b 5.57c 18.2b 21.5a 9.8c
Plotto et al. (2010)IV
April 2008 June 2008
Healthy HLB-SY Healthy HLB-SY
3.78 3.68 4.37 4.27
0.89 1.05 0.42 0.46
14.5 14.7 12.0 13.2
16.2 14.1 28.7 28.4
Liao and Burns, (2012)V
April 2009 Healthy HLB-AS HLB-SY
- 0.85b 0.85b 0.91a
11.6a 11.2a 9.3b
13.5a 13.1a 10.2b
Slisz et al. (2012)IV
May 2007 June 2007
Healthy HLB-AS Healthy HLB-AS HLB-SY
-
0.54 0.52 0.40 0.38 0.69
10.6 9.6
10.8 9.7 6.9
19.5 18.5 27.3 25.7 10.1
Raithore et al. (2015)III
April 2009
Healthy HLB-SY
4.17a 3.81a
0.62b 1.14a
12.2a 11.6a
19.7a 10.2b
Massenti et al. (2016)III
March + May 2013
Heatlhy HLB-AS HLB-SY
- 0.72b 0.75b 1.22a
12.4a 12.2a 8.5b
11.0a 10.4b 4.5c
Dala Paula et al. (2017b)VI
March 2013 Healthy HLB-SY
4.35a 3.86b
0.72b 0.94a
10.5a 9.6b
14.6a 10.1b
Leg.: TA: titratable acidity; SSC: solid soluble content; FJ: filtered juice; JWP: juice with pulp; AS: asymptomatic; SY: symptomatic; 1Blend of oranges harvested at Sep. 2004, Jul. and Oct 2005, and Aug. 2007; Values from the same reference with the same capital letter within columns do not differ in harvest time and values with the same small letter within columns do not differ in disease status, according to statistical analysis ( IFisher’s test significant difference test at P = 0.05; IIt test with the probability of error estimated to be lower than 0.000; IIIANOVA and Tukey’s test P ≤ 0.05; IVnot applicable; VDuncan’s multiple range test P<0.01; VIANOVA and Tukey’s test P ≤ 0.05 for SSC, and P ≤ 0.001 for TA and SSC/TA).
75
Table 4. Physicochemical characteristics of Hamlin orange juice made with
healthy fruit and fruit at different stages of HLB infection.
Reference
Orange juice sample Physicochemical characteristics
harvest time status or conditions
pH TA (g.100 mL-1)
SSC (°Brix)
SSC/TA
Hamlin orange juice
Bassanezi et al. (2009)I
Fruits of different harvests1
HLB-AS HLB-SY
- 0.76a 0.91b
9.6a 8.9b
13.1a 10.7b
Baldwin et al. (2010)II
December 2007 February 2008
Healthy HLB-AS Healthy HLB-SY
-
0.49Aa 0.50Aa 0.59Aa 0.50Aa
7.8Ba 7.6Ba
11.6Aa 10.4Ab
16.0Ba 15.3Ba 19.8Ab 22.0Aa
Plotto et al. (2010)III
February 2008
Healthy HLB-SY
4.19 4.17
0.50 0.52
11.9 11.4
23.8 22.1
Liao and Burns, (2012)IV
December 2007 Healthy HLB-AS HLB-SY
- 0.75a 0.80a 0.78a
11.3a 11.5a 9.1b
15.1a 14.3ab 11.7b
Raithore et al. (2015)V
January 2009 Healthy HLB-SY
4.22a 4.22a
0.52a 0.52a
11.4a 11.3a
21.7a 21.7a
Leg.: TA: titratable acidity; SSC: solid soluble content; AS: asymptomatic; SY: symptomatic; 1Blend of oranges harvested at Jul. 2007, Jun. and Jul. 2008. Values from the same reference with the same capital letter within columns do not differ in harvest time and values with the same small letter within columns do not differ in disease status, according to statistical analysis (It test with the probability of error estimated to be lower than 0.000; IIFisher’s test significant difference test at P = 0.05; IIInot applicable; IVDuncan’s multiple range test P<0.01; VANOVA and Tukey’s test P ≤ 0.05).
6.1.3 Sugars and organic acids
The results found for glucose in Valencia orange juice due to HLB infection
status were not consistent enough to establish an observable trend. Two of
three studies reported an increase of glucose in symptomatic juice, CLas (+),
compared to healthy juice, while one reported a decrease. In two different
studies, asymptomatic and healthy orange juice showed similarities in glucose
content; however certain harvests (May and June 2007) had higher glucose
contents in healthy juice compared to asymptomatic juice. For Hamlin juice,
there is one study comparing asymptomatic and healthy juice, from two different
harvest times, in which all of the samples showed a decrease of glucose in
asymptomatic juice compared to healthy juice (Table 5).
Changes in fructose due to HLB infection status also do not follow a clear
pattern. Fructose contents can either increase or decrease in symptomatic
orange juice. Between healthy and asymptomatic juices, the content is
generally similar. On the other hand, sucrose and total sugar contents decrease
in asymptomatic and, more notably, in symptomatic juices of Valencia and
76
Hamlin oranges (Tables 5 and 6), which would reflect the altered carbohydrate
transport in these infected oranges (CHIN et al., 2014). Asymptomatic and
healthy orange juice can have sucrose contents approximately 2.5 times higher
than that of symptomatic juice (SLISZ et al., 2012).
For individual organic acids, the majority of the studies reported similar
citric and ascorbic acid levels in healthy and asymptomatic orange juice, CLas
(+). However, symptomatic orange juice generally has a higher content of citric
acid and a lower content of malic acid compared to healthy juice (Tables 5 and
6). Typically, changes in individual and total sugar contents are more
pronounced in Hamlin than in Valencia orange juice (BALDWIN et al., 2010).
6.1.4 Secondary metabolites
Oranges are an important source of secondary metabolites which promote
human health, particularly flavonoids, limonoids, hydroxycinnamic acids and
polyamines. Many secondary metabolites result from the interaction between
the plant and its environment and are induced by biotic and abiotic elicitation.
Changes in the levels of certain classes of secondary metabolites are frequently
due to stress conditions in plants. In addition to stress conditions, these
compounds are influenced by many factors, such as: type of cultivar, cultivating
methods, degree of ripeness, and processing and storage conditions (SUDHA &
RAVISHANKAR, 2002; RAMAKRISHNA & RAVISHANKAR, 2011; CHIN et al.,
2014).
77
Table 5. Sugars and acids of Valencia orange juice made with healthy fruit and fruit at different stages of HLB infection.
Leg.: FJ: filtered juice; JWP: juice with pulp; AS: asymptomatic; SY: symptomatic. Values from the same reference with the same capital letter within columns are not significantly by different harvest time and with the same small letter within columns are not significantly by disease status following statistical analysis (IFisher’s test significant difference test at P = 0.05; II Duncan’s multiple range test P<0.01; IIIP-values represent comparisons within harvest *p < 0.05; **p < 0.001; IVANOVA and Tukey’s test P ≤ 0.05; Vnot applicable; VIANOVA and Tukey’s test P ≤ 0.05 for glucose, total sugars and malic acid, and P ≤ 0.01 for sucrose, fructose and citric acid).
Reference Orange juice sample Sugars (g.100 mL-1) organic acids (g.100 mL-1)
harvest time status or conditions glucose fructose sucrose total sugars citric acid malic acid
Plotto et al. (2008)I July 2006
Healthy FJ HLB FJ Healthy JWP HLB JWP
2.8a 2.8a 2.6ab 2.5b
1.9a 1.9a 1.8ab 1.7b
4.3a 4.1a 4.1ab 3.7b
-
0.52a 0.45b 0.48ab 0.40c
0.13a 0.10b 0.11b 0.09c
Baldwin et al. (2010)I
March 2007 April 2007 May 2007 June 2007
Healthy HLB-AS Healthy HLB-AS Healthy HLB-AS Healthy HLB-AS
1.9Aa 1.9Aa 1.9Aa 1.7Aa 2.0Aa 1.8Ab 2.0Aa 1.8Ab
1.9Aa 1.9Aa 2.0Aa 1.8Aa 2.0Aa 1.9Aa 2.0Aa 1.9Aa
4.9Ba 4.7Aa 5.2ABa 4.4Ab 5.5Aa 4.8Ab 5.6Aa 4.8Ab
8.7Ba 8.6Aa 9.1ABb 8.0Ab 9.5ABa 8.5Ab 9.7Aa 8.4Ab
- -
Liao and Burns (2012)II April 2009 Healthy HLB-AS HLB-SY
- - - 7.1a 6.8a 1.8b
- -
Slisz et al. (2012)III
May 2007 June 2007
Healthy HLB-AS Healthy HLB-AS HLB-SY
1.38 1.30 1.37 1.24 1.12
1.70 1.57 1.70 1.64 1.47
4.13 3.71 4.64
3.90** 1.54
-
0.64 0.57 0.47 0.38 0.91
0.26 0.23 0.26 0.22* 0.18
Raithore et al. (2015)IV April 2009
Healthy HLB-SY
2.16a 2.69a
2.30a 2.68a
4.95a 3.39b
- 0.53b 1.40a
0.17a 0.12b
Baldwin et al. (2017)V
March-April 2013 2014 2015
HLB HLB HLB
1.4 1.9 1.9
1.9 2.2 2.2
3.9 3.8 3.7
7.2 7.9 7.8
0.42 0.80 0.67
0.13 0.18 0.61
Dala Paula et al. (2017b)VI
March 2013 Healthy HLB-SY
2.0b 2.3a
2.3b 2.7a
5.6a 4.2b
10.0a 9.0b
0.84b 1.41a
0.14a 0.11b
78
Table 6. Sugars and acids of Hamlin orange juice made with healthy fruit and fruit at different stages of HLB infection.
Leg.: AS: asymptomatic; SY: symptomatic. Values from the same reference with the same capital letter within columns are not significantly by different harvest time and with the same small letter within columns are not significantly by disease status following statistical analysis (IFisher’s test significant difference test at P = 0.05; IIANOVA and Tukey’s test P ≤ 0.05 for glucose, total sugars and malic acid, and P ≤ 0.01 for sucrose, fructose and citric acid).
Reference
Orange juice sample Sugars (g.100 mL-1) organic acids (g.100 mL-1)
harvest time status or
conditions glucose fructose sucrose
total
sugars citric acid malic acid
Baldwin et al. (2010)I December
2007
February
2008
Healthy
HLB-AS
Healthy
HLB-AS
1.5Ba
1.3Bb
2.2Aa
1.8Ab
1.5Ba
1.4Ba
2.2Aa
1.8Ab
3.9Ba
3.2Bb
5.4Aa
4.0Ab
7.0Ba
6.0Bb
9.8Aa
7.6Ab
- -
Raithore et al.
(2015)II
January
2009
Healthy
HLB-SY
2.9a
2.7a
3.0a
2.7a
5.4a
4.7a -
0.53a
0.55a
0.16a
0.17a
79
Generally, higher concentrations of phenolic compounds are found in
sprouts and seedlings compared to mature plants, consistent with the notion
that plant phenolics provide a degree of protection against predation
(DREWNOWSKI & GOMEZ-CARNERO, 2000). Similarly, there is an increase
of phenolic compound levels in orange juice and leaves from trees infected with
CLas (DAGULO et al., 2010; HIJAZ et al., 2013; KIEFL et al., 2017). Flavonoid
contents, particularly narirutin and hesperidin, are higher in the peel, pulp and
juice of HLB symptomatic fruit (MASSENTI et al., 2016; KIEFL et al., 2017)
compared to the respective healthy fruit parts. The pulp of HLB symptomatic
Valencia oranges from two different harvest times (March and May 2013)
showed an increase of 147.9% and 16.9%, in narirutin, respectively, and an
increase of 85.5% and 94.1% in hesperidin, respectively, compared to the
corresponding healthy fruit pulp (MASSENTI et al., 2016). Juice from
symptomatic Valencia oranges harvested in March 2013, contained higher
amounts of tangeretin (> 4x), nobiletin (> 2x), heptamethoxyflavone (> 1.5x),
diosmin (> 2x), didymin (> 1.5x), 6,8-di-C-glucosyl apigenin (> 1.5x), nomilin (>
20x), limonin (> 7.5x) and limonin glucoside (> 1.5x) compared to healthy juice
(DALA PAULA et al., 2017b). The polymethoxyflavone, tangeretin, is also high
in symptomatic Valencia and Hamlin juice (KIEFL et al., 2017).
Juice made with asymptomatic, CLas (+), and healthy, CLas (-), Hamlin
oranges harvested in February and April 2008, respectively, had similar limonin,
nomilinic acid glucoside, nomilin glucoside, narirutin, limonin glucoside,
narirutin-4’-glucoside, feruloyl-putrescine, 6,8-di-C-glucosyl apigenin, alkaloid
and hydroxycinnamic acid contents. Healthy and asymptomatic Valencia
oranges differed in nomilin glucoside and nomilin levels in their juice (BALDWIN
et al., 2010).
Juices made with asymptomatic and, especially, symptomatic oranges,
CLas (+), contain high levels of nomilin and limonin. Both, nomilin and limonin
are known to provide bitterness in citrus fruit and its juice, however their levels
in HLB orange juice are usually below the threshold for bitter perception (DEA
et al., 2012) and, in fact, only symptomatic oranges have their taste
compromised (BALDWIN et al., 2010; PLOTTO et al., 2010; SLISZ et al., 2012;
CHIN et al., 2014; RAITHORE et al., 2015; DALA PAULA et al., 2017b). This
80
suggests that there may be other compounds involved with the bitter taste in
CLas (+) symptomatic orange juice.
6.1.5 Amino acids and bioactive amines
The accumulation of proline, arginine and the branched chain amino acids
is expected in plants subjected to conditions which induce stress, such as
drought, high salinity and acidity, high incidence of light, high concentration of
heavy metals in the soil, changes in temperature, as well as in response to
biotic stress, such as plant diseases (RAI, 2002; SHARMA & DIETZ, 2006;
SLISZ et al., 2012; MALIK et al., 2013). However, the amino acids: alanine,
arginine, isoleucine, leucine, proline, threonine, and valine are found in lower
concentrations in symptomatic orange juice, CLas (+). In symptomatic Valencia
and Hamlin orange juices, the concentrations of asparagine and phenylalanine
are over 2 times higher and histidine content is also increased (SLISZ et al.,
2012; CHIN et al., 2014). A suggested explanation for this trend is that CLas
may have inhibited the tree’s defense mechanism which, in turn, reduced the
action of proline dehydrogenase, an enzyme responsible for the activation of
the biosynthetic pathways of proline from ornithine and glutamate. Thus, the
levels of this amino acid could not increase (SLISZ et al., 2012).
The changes in amino acid contents due to infection status in orange trees
allowed the use of their levels as biomarkers to identify early detection of
asymptomatic trees. The differences of the local harvest and cultivars did not
compromise the use of metabolite composition in the discernment of HLB
infection status in the oranges (CHIN et al., 2014).
Hamlin and Valencia symptomatic oranges, CLas (+), show high contents
of synephrine, an aromatic amine, however asymptomatic and healthy juices
have similar contents (SLIZS et al., 2012; CHIN et al., 2014). In plants,
putrescine is a necessary diamine precursor of polyamines (spermidine and
spermine) synthesis and its increase is usually associated with environmental
stress in plants (COELHO et al., 2005; GLÓRIA, 2006; SHARMA & DIETZ,
2006); however, putrescine content is not affected in symptomatic juice (CHIN
et al., 2014). On the other hand, feruloyl putrescine, a conjugate of putrescine
and ferulic acid, is found at high concentrations in symptomatic Hamlin juice
81
compared to asymptomatic and healthy juice. The same trend does not seem to
be observed in Valencia oranges (BALDWIN et al., 2010).
6.2 Effects on sensory characteristics
The aroma of orange juice is due to the complex combination of various
flavor and odor components. Alcohols, aldehydes, esters, ketones,
hydrocarbons, sugars and secondary metabolites, such as phenolic compounds
and bitter limonoids have been investigated in orange juice affected by CLas
(PLOTTO et al., 2008; 2010; 2017; BALDWIN et al., 2010; 2012a; DAGULO et
al., 2010; MASSENTI et al., 2016; DALA PAULA et al., 2017b). Some taste
descriptors have been used to describe the effects of HLB infected oranges
since the 1970s, for example, bitter and salty (McCLEAN & SCHWARZ, 1970;
MOLL & VAN VUUREN, 1977; BALDWIN et al., 2010; PLOTTO et al., 2010;
RAITHORE et al., 2015).
Years later, after HLB had been reported in both South and North
America, some researchers began to take a deeper look into the sensory
effects of orange juice caused by HLB. Recently, with the evolution of sensory
analysis as an increasingly important component of food science and the
increased interest on the topic, CLas (+) orange juice has been associated with
several negative effects regarding taste (astringency, tingling, harshness,
bitterness, metallic-taste, low sweetness, saltiness/umami, musty,
sourness/fermented, pungent/peppery, low citrusy taste) (Tables 7 and 8),
usually due to an imbalance in the chemical composition (BALDWIN et al, 2010;
2012b; PLOTTO et al., 2010; RAITHORE et al., 2015; DALA PAULA et al.,
2017b; KIEFL et al., 2017).
82
Table 7. Sensorial descriptors ascribed to Huanglongbing in Valencia orange
juice
Sensorial descriptor* Harvest time Juice specifications Reference
Acidic Jul. 2006, Apr. 2008 frozen juice with pulp and filteredI, hand-squeezed juice II
1; 4
Astringent Jun. 2008; Mar. 2013 commercially processed juiceIII 2; 5
Bitter/slight bitter Jun. 2008; Mar. 2013 commercially processed juice 2; 5
Bland Jun. 2008 commercially processed juice 2
Burning Mar. 2013 commercially processed juice 5
Fermented Jul. 2006 frozen juice with pulp and filtered 1
Grapefruit-like flavor Apr. 2008, Jun. 2008; Mar. 2013
commercially processed juice 2; 5
Green flavor Mar. 2013 commercially processed juice 5
HLB-bitter Monthly basis during the season 2014 and 2015
hand-squeezed juice 4
Less fruity non-citrus flavor**
Mar; 2013 commercially processed juice 5
Less orange flavor** Mar. 2013 commercially processed juice 5
Less sweet** Apr. 2008, Mar. 2013 commercially processed juice 2; 5
Metallic Jun. 2008; Apr. 2009 commercially processed juice 3
Off flavor Apr. 2008 commercially processed juice 2
Overripe Jul. 2006 frozen juice with pulp and filtered 1
Peel oil Apr. 2008, Jun. 2008; Mar. 2013
commercially processed juice 2; 5
Salty/umami Apr. 2009; Mar. 2013 commercially processed juice 3; 5
Sharp Apr. 2008, Jun. 2008 commercially processed juice 2
Sour Apr. 2008, 2009; Mar 2013 commercially processed juice 2; 3; 5
Stale Mar. 2013 commercially processed juice 5
Sweeter** Apr. 2008 commercially processed juice 2
Tangy Apr. 2008 commercially processed juice 2
Tingly Apr. 2009 commercially processed juice 3
Typical HLB flavor Mar. 2013 commercially processed juice 5
Unidentifiable different flavor
Jun. 2008 commercially processed juice 2
Weak in taste Jul. 2006 frozen juice with pulp and filtered 1 *The list of sensorial descriptors includes commentaries realized by the panel during sensory evaluations and attributes significantly higher in asymptomatic or symptomatic orange juice, CLas (+), compared to healthy juice (control); **in comparison with control juice - healthy orange juice, CLas (-); ***According to the authors, HLB-bitter refers to a long-lasting metallic, astringent and harsh taste. Ifrozen juice thawed overnight served with the pulp and without pulp. Juice was filtered then flash pasteurized at 71 °C for 10 s and immediately cooled then served; IIoranges were hand juiced and lightly pasteurized using at 71 °C for 15 s, and frozen at - 20 °C; IIIfruit were extracted using a commercial JBT 391 single head extractor with premium juice extractor settings, and pasteurized under simulated commercial conditions (1.2 L/m, 8 to 10 s hold time, 83 to 90 °C). Leg.: 1PLOTTO et al., 2008; 2PLOTTO et al., 2010; 3RAITHORE et al., 2015; 4KIEFL et al., 2017; 5DALA PAULA et al., 2017b.
83
Table 8. Sensorial descriptors ascribed to Huanglongbing in Hamlin orange
juice
Sensorial descriptor*
Harvest time Juice specifications Reference
Astringent Feb. 2008; commercially processed juice 1
Bitter Dec. 2007; Feb. 2008; Jan. 2009
hand-squeezed juice, commercially processed juice
1; 2
Cooked Jan. 2009 commercially processed juice 2
Earthy Feb. 2008; commercially processed juice 1
Fatty Feb. 2008 commercially processed juice 1
Fermented Feb. 2008; commercially processed juice 1
Grapefruit-like Dec. 2007; Feb. 2008; Jan. 2009
hand-squeezed juice, commercially processed juice
1; 2
HLB bitter*** Monthly basis during the season 2014 and 2015
hand-squeezed juice 3
Less freshness Feb. 2008 commercially processed juice 1
Less orange flavor** Feb. 2008 commercially processed juice 1
Less sweet** Feb. 2008; commercially processed juice 1
Metallic Feb. 2008; commercially processed juice 1
Musty Feb. 2008; commercially processed juice 1
Overripe Jan. 2009 commercially processed juice 2
Peel oil/citrus oil Dec. 2007; Feb. 2008; Jan. 2009
hand-squeezed juice, commercially processed juice
1; 2
Peppery Feb. 2008; commercially processed juice 1
Pungent Feb. 2008 commercially processed juice 1,
Salty/umami Feb. 2008 commercially processed juice 1
Sharp Dec. 2007; hand-squeezed juice 1
Sour Dec. 2007; Feb. 2008; Jan. 2009
hand-squeezed juice, commercially processed juice
1; 2
Sour milk Dec. 2007; hand-squeezed juice 1
Sulfury Jan. 2009 commercially processed juice 2
Tingly Feb; 2008 commercially processed juice 1 *The list of sensorial descriptors includes commentaries realized by the panel during sensory evaluations and attributes significantly higher in asymptomatic or symptomatic orange juice, CLas (+), compared to healthy juice (control); **in comparison with control juice - healthy orange juice, CLas (-); ***According to the authors, HLB-bitter refers to a long-lasting metallic, astringent and harsh taste. Ifrozen juice thawed overnight served with the pulp and without pulp. Juice was filtered then flash pasteurized at 71 °C for 10 s and immediately cooled then served; IIoranges were hand juiced and lightly pasteurized using at 71 °C for 15 s, and frozen at - 20 °C; IIIfruit were extracted using a commercial JBT 391 single head extractor with premium juice extractor settings, and pasteurized under simulated commercial conditions (1.2 L/m, 8 to 10 s hold time, 83 to 90 °C). Leg.: 1PLOTTO et al., 2010; 2RAITHORE et al., 2015; 3KIEFL et al., 2017;
According to the chemical and physicochemical changes observed in
orange juice as the season progresses, the effects of HLB on sensory
characteristics are more pronounced in symptomatic juice made from oranges
harvested earlier in the season (MCCLEAN & SCHWARZ, 1970; RAITHORE et
84
al., 2015). In addition, there is a large variation in the effect of CLas on the
quality of orange juice due to cultivar, maturity, and individual tree. Comparing
Hamlin and Valencia, the off-flavor resulting from the disease is generally more
noticeable in Hamlin oranges. Juice made with these symptomatic, CLas (+)
oranges generally has the most off-flavors, commonly described as “bitter”,
“sour” and “sour/fermented”. On the other hand, for certain harvests,
symptomatic Valencia orange juice is no different from its healthy juice. When
they are different, the HLB juice is described as “bitter” or “off-flavor” (PLOTTO
et al., 2010).
The HLB off-flavor is so pronounced that processing healthy fruits with
infected ones can affect the sensory quality of the orange juice, negatively
impacting the citrus industry (BASSANEZI et al., 2009). Juice from CLas (+)
symptomatic fruit can be blended with juice from CLas (-) fruit, up to 25%
symptomatic juice, without being perceived as off-flavored. Considering the
increased spread of HLB in the US, this may be considered valuable
information for the citrus industry and can help maintain commercial
acceptability of orange juice in regions where HLB is prevalent (RAITHORE et
al., 2015).
HLB-infected juice with lower sugar contents, an altered volatile profile and
sometimes higher acids, tastes unpleasant. In addition to these components,
the orange fruit also contains some secondary metabolites including different
classes of flavonoids (flavanone, flavone, polymethoxyflavone, hydroxycinnamic
acid derivatives, coumarins, and anthocyanins) and triterpenoids which
influence taste. Limonin and nomilin exist in glycosides forms being tasteless,
and aglycone forms. The aglycone of the triterpenoids limonin and nomilin are
well known to be bitter and/or metallic in taste. Interestingly, the levels of bitter
limonoids were either at or below reported thresholds (the concentration at
which a compound can be detected); yet, panelists were able to detect a bitter
and metallic flavor in symptomatic CLas (+) orange juice. Further research
showed that the threshold for the detection of bitterness in orange juice was
lowered if the two bitter limonoids (limonin and nomilin) were present together,
indicating synergy between them (HASEGAWA, 1983; DEA et al., 2013).
There is a strong correlation between limonoid and flavonoid
concentrations and the off-flavor and quality of the oranges (KIEFL et al., 2017).
85
It is known that commercial polymethoxyflavone (PMF) preparations from citrus
peel possess a bitter taste. Nobiletin and tangeretin were reported as the two
main bitter PMFs present in citrus peel, with tangeretin bitterness determined to
be 2-3 times higher than nobiletin by sensory analysis and 3-4 times higher
using a receptor-based method in vitro (BATENBURG et al., 2016). Recently,
hesperidin was also suggested to be a key compound of HLB induced orange
juice off-flavor, indirectly acting as a taste modulator enhancing unacceptably
harsh, metallic and bitter characteristics (KIEFL et al., 2017). Additionaly, in
hesperidin can contribute to the formation of sediments which result in
undesirable cloudiness in orange juice (GATTUSO et al., 2007).
Unlike other tastes, the detection thresholds for bitterness are generally
extremely low. For example, the bitter quinine was detected at 25 μmol/L.
Furthermore, the bitter after-taste can also be more prolonged than others
(DREWNOWSKI & GOMEZ-CARNEROS, 2000). Bitterness is appreciated in
some kinds of food and beverages, such as bitter chocolate and coffee
however, it greatly reduces the acceptability of orange juice (PLOTTO et al.,
2008; 2010).
The polyphenol contained in foods and beverages are classified into many
classes, from small molecules, such as hydroxycinnamic acids, to big polymers,
such as lignin. This vast group of compounds may be responsible for the
bitterness and astringency of many foods and beverages. Astringency, a typical
mouthfeel, is perceived as a long-lasting trigeminal sensation in the oral cavity
which may be due to a reaction between dietary polyphenols and proteins in the
mouth and saliva and can be classified into sub qualities such as velvety,
grainy, drying or puckering (DREWNOWSKI & GOMEZ-CARNERO, 2000;
HUFNAGEL & HOFMANN, 2008;). In general, phenolics of lower molecular
weight are bitter, while higher molecular weight polymers tend to be more
astringent (DREWNOWSKI & GOMEZ-CARNEROS, 2000). However, this
assumption is not consistently applicable. For example, the phenolic
compounds of black tea were separated into three fractions according to the
different molecular weights and then described by a sensory panel. The fraction
containing low molecular weight compounds was described as the most
astringent and represented the typical taste profile of the black tea
(SCHARBERT et al., 2004).
86
6.3 Effect on the levels and profile of volatile compounds
Ten odor-active compounds were chemically identified in pasteurized
orange juice and their odors were described utilizing multidimensional gas
chromatography coupled with olfactometry and mass spectrometry. Grassy and
plastic-like odors were attributed to α-pinene; fruity and sweet odors to ethyl
butanoate; grassy and green odors to hexanal; citric, mint and sweet odors to
heptanal, methyl hexanoate and D-limonene; fresh, lemony, green, fatty and
bug odors to octanal; flower and lemon odors to linalool; and mint, green, fruity
and citrus odors to α-terpineol and citral. Other than these odor descriptions,
other unidentified compounds were described as mushroom, spicy, wood,
cheese, citric and caramel odors (MASTELLO et al., 2015). Some of these
descriptors were very similar to those obtained from the taste dilution
fractionation test of phenolic compounds extracted by fast centrifugal partition
chromatography in healthy and symptomatic CLas (+) Valencia orange juice
(DALA PAULA et al., 2017a; 2017b), as well as the observations recorded by
the panel during the sensory evaluation of differences between healthy and
asymptomatic Hamlin orange juice (PLOTTO et al., 2010). However, unlike
Mastello et al. (2015), in the study of Valencia orange juice, the authors only
evaluated non-volatile compounds.
Regarding other chemical and physicochemical attributes, the harvest date
is a more influential factor in changing the volatile contents of orange juice
compared to infection status (BALDWIN et al., 2010). However, HLB infection
significantly affects the levels of odor active compounds in orange peel oil
(KIEFL et al., 2017) and orange juice. Symptomatic, Clas (+), Valencia juice
made with oranges harvested from December to May in 2007/2008 showed
higher contents of 26 volatile compounds and lower contents of the following 9
compounds: ethyl butanoate, ethyl hexanoate, 1-Octen-3-ol, β-selinene, ethyl-3-
hydroxyhexanoate, valencene, α-selinene and β-Ionone) compared to healthy
juice (DAGULO et al., 2010).
Among the 22 volatile compounds identified in juice made with healthy and
asymptomatic, CLas (+), Hamlin oranges harvested in different months in 2007
and 2008, only two volatiles showed significant differences due to infection
87
status. The samples had higher contents of ethyl hexanoate and lower contents
of sabinene compared to control juice. Homemade Valencia juice made with
asymptomatic oranges, CLas (+), harvested in different months of 2007 showed
significant differences in 9 compounds. The samples had lower contents of
octanal, decanal, trans-2-hexenol, valencene and ethyl butanoate and higher
contents of 2-methylpropanol, cis-3-hexenol, sabinene and ethyl hexanoate
compared to control juice. Commercial Valencia juice made with asymptomatic
oranges harvested in various months of 2008 showed significant differences in
two compounds, the samples had higher contents of ethanol and lower contents
of ethyl acetate compared to the control (BALDWIN et al., 2010). These results
suggest different levels of volatiles due to different harvest times, types of
processes used to prepare the orange juice (BALDWIN et al., 2012a) and HLB
infection status. It is important to emphasize that, generally, asymptomatic
orange juice is similar to healthy orange juice.
Orange juice made with HLB symptomatic fruit, CLas (+), has higher levels
of α- and β-sinensal (37 and 59%, respectively), linalool (20%), and numerous
limonene and linalool degradation compounds compared to healthy orange
juice. On the other hand, healthy orange juice has higher levels of octanal
(22%), decanal (6%), undecanal (6%), 6-methyloctanal (23%), ethyl butanoate
(163%), ethyl hexanoate (169%), ethyl octanoate (57%), nootkatone (128%),
valencenes (51%), (Z)-4decenal (38%) and (E,E)-2,4-decadienal (19%)
compared to HLB orange juice. The difference in ethyl-butanoate concentration
was more noticiable in healthy than in HLB orange juice. This ethyl ester
imparts fruity and sweet odors in healthy orange juice (KIEFL et al., 2017).
6.4 Huanglongbing control and mitigation of its symptoms
To this date, there is no cure for HLB and the prevention of the spread of
the disease relies primarily on controlling psyllid populations (STANSLY et al.,
2010; MARTINI et al., 2016). Currently, preventing CLas from infecting healthy
citrus trees is much easier than trying to eradicate or control it. The control of
HLB is still difficult, especially if the bacteria are widespread and their vectors
are well established. The most effective control strategy has been to remove the
trees infected with HLB in an area and then replant with HLB-free trees
88
(ABDULLAH et al., 2009). Other common management strategies include
chemical insect control and nutritional spray applications (ALBRECHT et al.,
2012).
Florida growers have been using foliar nutritional spray products that
often contain micro-nutrients and compounds that supposedly activate systemic
acquired resistance to help boost tree health and defense response
(MASUOKA et al., 2011; BALDWIN et al., 2012b). The benefits of this approach
to disease management in the field are questionable because the inoculums
remain after application. Unfortunately, this method of managing HLB potentially
contributed to the propagation of the disease in Florida because many Floridian
farms stopped eliminating their affected trees. Unless the vectors are thoroughly
controlled, the spread of HLB to other orchard trees and neighboring farms is
inevitable (TIMMER et al., 2011; GOTTWALD et al., 2012).
In an evaluation of nutritional spray treatments, Hamlin oranges from
trees that received the treatment had the same off-flavor as oranges from trees
that did not receive the treatment, whereas Valencia oranges were notably
sweeter. The nutritional treatments did not consistently result in less pathogen
DNA for either cultivar (BALDWIN et al., 2012b). The implementation of
combined nutrient programs and insecticide treatments has been studied and
the results suggest that the beneficial effect of increased orange juice quality
may have been cumulative, only manifesting later on during the third year
(BALDWIN et al., 2017; PLOTTO et al., 2017).
7. Final considerations
HLB affects the physicochemical characteristics of orange juice.
Symptomatic juice tends to have high TA, low SSC and SSC/TA, while
asymptomatic juice tends to be similar to healthy juice. In general, HLB causes
a decrease in sucrose, total sugar and malic acid contents while ascorbic acid
does not seem to be significantly affected by the disease. On the other hand,
levels of citric acid, bitter limonoids (limonin and nomilin), hydroxycinnamic
acids, flavonoids, particularly tangeritin, nobiletin, narirutin, hesperidin, diosmin
and didymin are higher in HLB symptomatic juice compared to healthy juice.
Thus, there is a strong correlation between the limonoid and flavonoid
89
concentrations and the off-flavor and quality of the oranges. The amino acid
contents, alanine, arginine, asparagine, histidine, isoleucine, leucine,
phenylalanine, proline, threonine and valine are altered by HLB. Additionally,
symptomatic Hamlin orange juice has high synephrine and feruloyl putrescine
levels.
Regarding the typical HLB-off flavor in orange juice, the loss of
sweetness can generally be explained by lower sucrose levels, total sugar
levels and SSC, along with higher citric acid levels. The sensory descriptors of
sourness, umami and tingling were correlated with some volatile compounds,
and with tangeretin and nobiletin. The sourness can be partially explained by
higher TA and citric acid content generally found in HLB orange juice. Elevated
levels of limonin and nomilin, which occur in juice made with oranges harvested
from symptomatic and/or asymptomatic HLB infected trees, are partially
responsible for the typical HLB-bitterness. These two liminoids have a
synergistic effect which decreases their perception and identification thresholds
in orange juice. Furthermore, there is evidence indicating that other compounds,
possibly hydroxycinnamic acids, are involved with the typical HLB-bitterness.
Additionally, the lowest SSC, SSC/TA and sugar contents typically perceived in
symptomatic orange juice, CLas (+) can reinforce the perception of bitterness.
There are relatively few published papers evaluating the effects of HLB
on orange juice’s chemical, physicochemical and, especially its sensorial
qualities and most of the research available was performed using Valencia
oranges, followed by Hamlin samples. The evaluation of the effects of HLB is
complex due to various factors that can obscure them. Thus, subsequent
research is required to better understand the effects of HLB on orange juice and
to identify solutions for its negative sensory attributes.
90
CAPÍTULO III - ACTIVE TASTE COMPOUNDS IN JUICE MADE
FROM ORANGES SYMPTOMATIC OF HUANGLONGBING (HLB)
GREENING DISEASE
ABSTRACT
Citrus greening disease, also known as Huanglongbing (HLB),
compromises the quality of citrus fruit and juice, causing increased bitterness
and metallic taste, astringency and a burning mouthfeel. The chemical basis
responsible for these changes remains largely unknown other than the roles of
the bitter limonoids, limonin and nomilin, and of flavonoids that may cause
astringency. A combination of chemical and sensory analyses was used to
identify bitter components in orange juice made from oranges symptomatic for
HLB, and comparisons were made with juice made with healthy fruit. The
results showed that there were statistical differences in pH, total acidity (TA),
soluble solids content (SSC), SSC/TA, total sugars, organic acids, secondary
metabolites and sensory characteristics between healthy and HBL-affected
orange juices. Nonvolatile juice compounds were fractionated using fast
centrifugal partition chromatography and semipreparative HPLC. Some
fractions were described as bitter, but did not contain limonoids,
polymethoxylated flavones (PMF) or hesperidin, and instead they were
overwhelmingly composed of hydroxycinnamates, indicating that these
compounds might also be involved with this sensory attribute.
KEYWORDS: Huanglongbing. Bitterness. Hydroxycinnamic acids. Limonoids.
Orange juice.
Artigo submetido a LWT – Food Science and Technology
Autores: DALA PAULA, B.M.; RAITHORE, S.; MANTHEY, J.A.; BALDWIN,
E.A.; BAI, J.; ZHAO, W.; GLÓRIA, M.B.A.; PLOTTO, A.
91
1. INTRODUCTION
Worldwide citrus production has been adversely affected by citrus
greening disease or Huanglongbing (HLB), associated with the presence of the
gram-negative bacteria Candidatus Liberibacter asiaticus (Clas) transmitted by
the Asian Citrus psyllid Diaphorina citri (BOVÉ, 2006). The HLB was first
reported in 1919 in Southern China, and has now spread throughout more than
40 countries in Africa, Asia and the Americas (South and North) (UF/IFAS
Extension, 2013). The first case of HLB in the Western Hemisphere was
reported in the State of São Paulo, Brazil, in March 2004 (TEIXEIRA et al.,
2005a), and a year later, in August 2005, HLB was confirmed in South Florida,
USA (BOVÉ, 2006). Now, HLB is present in all of the Florida citrus-growing
counties, and the production of oranges for processing fell from 140 million
boxes in 2005-2006 to less than 70 million boxes in 2016-2017 (UF/IFAS
Extension, 2013; USDA NASS, 2016). Texas and Arizona also have HLB which
is affecting their production as well (USDA/FAS, 2017).
In addition to causing the deterioration and death of citrus trees, HLB has
a negative impact on fruit quality and results in off-flavored orange juice. Since
90% of the oranges grown in Florida are juiced, the quality of the final product is
vital for competition in the global market. Juice produced from HLB-affected fruit
has been characterized as having negative attributes including sour, bitter,
salty, metallic, astringent, tingling, with bitter, astringent and burning aftertaste
(PLOTTO et al., 2010; 2017), purportedly resulting from changes in the
chemical composition of the disease-affected fruit (BASSANEZI et al., 2009;
BALDWIN et al, 2010; DAGULO et al., 2010; RAITHORE et al., 2015; KIEFL et
al., 2017).
In stress situations as caused by diseases such as HLB, plants respond
by accelerated synthesis of certain secondary metabolites. Several authors
observed higher bitter limonoids, sometimes higher acids, lower sugar contents,
and generally higher flavonoids in HLB-affected fruit compared to healthy fruit
(BALDWIN et al., 2010; DAGULO et al., 2010; PLOTTO et al., 2010;
MASSENTI et al., 2016). It has been shown that the negative taste effect is
caused by interactions of these various chemical classes rather than one single
component. The roles of reduced sugar and increased limonoids in bitter taste
92
are well understood (HOROWITZ & GENTILI, 1963; DREWNOWSKI &
GOMEZ-CARNEROS, 2000; DEA et al., 2013; BATENBURG et al., 2016). Dea
and co-authors (2013) showed how adding sucrose to orange juice spiked with
limonin and nomilin resulted in decreased bitterness induced by these
compounds. Similarly, spiking limonin at 10 mg.L-1 to Valencia juice with high
soluble solids content had little effect on bitterness contrary to spiking the same
amount of limonin to a low sugar Hamlin juice (KIELF et al., 2017). Adding to
the complexity is the synergism found between limonin and nomilin which
decreased the detection thresholds when combined together in orange juice
(DEA et al., 2013).
Until recently, focus on orange juice bitterness has been nearly
exclusively on limonoids, so it is not well documented whether other secondary
metabolites such as flavanone neohesperidosides (naringin, neohesperidin,
poncirin and neoeriocitrin) or polymethoxylated flavones - PMF (nobiletin and
tangeretin), also play any role or not. Batenburg et al. (2016) showed that
tangeretin and nobiletin were the main bitter components in citrus peel-derived
PMF preparations, with tangeritin 2-3 times more bitter than nobiletin. However,
in juice, these compounds occur at concentrations far below their detection
thresholds, making it unlikely that they directly contribute to orange juice
bitterness (KIEFL et al., 2017; PLOTTO et al., 2017). Kiefl et al. (2017)
attempted to demonstrate bitterness in orange juice by spiking with either
limonin, PMFs, poncirin and hesperidin, alone or in combination. They were
able to show an increase in bitterness from the mixture of all flavonoids plus
limonin, but it was not clear which specific flavonoids would contribute to any of
these complex taste descriptors.
Multiple words describe taste and flavor of orange juice from HLB-
affected fruit and suggest that changes in taste due to HLB are results of
complex alterations in chemical composition. Therefore, the objectives of this
study were to quantify the differences between healthy and HLB-affected
orange juice, and to identify sensory-active fractions in HLB-affected orange
juice extracts possessing bitter, astringent or harsh properties. This work will
contribute to potential identification of compounds responsible for the bitterness
(other than limonin, nomilin, tangeretin, and nobiletin) typical of HLB
93
symptomatic fruit and juice to potentially detect the presence of compounds that
mitigate off-flavors in HLB-affected orange juice.
2. MATERIAL AND METHODS
2.1 Juice samples
2.1.1 Sample preparation
‘Valencia’ oranges (Citrus sinensis (L.) Osbeck) were harvested from a
commercial grove in March 2013, from multiple healthy and HLB-affected trees.
The fruit were then separated into healthy controls and HLB-symptomatic fruit
(small green and lopsided, testing positive for CLas by qPCR), and juice was
extracted using a JBT Food Tech extractor system and pasteurized (BALDWIN
et al., 2012b) resulting in healthy control juice (COJ) and HLB juice (HLBOJ).
2.1.2 DNA extraction and qPCR detection of CLas from juice
DNA was extracted from 500 µL of orange juice using a modified CTAB
method (ZHAO et al., 2015; BALDWIN et al., 2017). Briefly, DNA quality
(260/280 and 260/230 ratio) and quantity were assessed by spectrophotometry
(Nano Drop, Thermo Scientific, Waltham, MA). CLas detection was
accomplished by qPCR. Specific primers targeting CLas 16S rRNA gene (Li
primers) (LI et al., 2006) or CLas hyv1 (LJ primers) (MORGAN et al., 2012)
were synthesized by Integrated DNA Technologies, Inc. (Coralville, IA). The
qPCR parameters were as follows: 95 °C for 10 minutes, followed by 40 cycles
at 95 °C for 15 seconds, and 60 °C for 1 minute, with fluorescence signal
capture at each stage of 60 °C. For SYBR® Green Real-Time PCR (with LJ
primers), the default Melt Curve (disassociation) stage is continued after the 40
cycles of PCR.
2.2 Chemical analysis of COJ and HLBOJ
2.2.1 Titratable acidity and soluble solids
For quality determination, solid soluble content (SSC) and titratable
acidity (TA) were determined prior to individual sugar and acid analyses. SSC
94
was determined by refractive index measured with a digital ATAGO PR-101
refractometer (Atago Co, Tokyo, Japan) and TA was calculated by titration of
10 mL of juice with 0.1 mol.L-1 NaOH to a pH 8.1 endpoint using an autotitrator
(Metler Toledo DL50, Columbus, OH, USA) (BALDWIN et al., 2017).
2.2.2 Total sugar, sucrose, glucose and fructose
Individual sugars were analyzed with a high performance liquid
chromatography (HPLC) system using a Perkin-Elmer Series 200 autosampler
and pump (Perkin-Elmer, Waltham, MA). Sample preparation was according to
Baldwin et al. (2012a), where juice samples were extracted with 80% (v/v)
aqueous ethanol, boiled for 15 min, cooled, and run through several levels of
filtration. The separation column was a Sugar-Pak™ I (10 µm, 6.5 x 300 mm)
(Waters, Milford, MA) operated at 90 °C in a CH-30 column heater and a TC-50
controller (FIAtron, Milwaukee, WI). Run conditions were an isocratic system of
0.001 mol.L-1 calcium ethylenediaminetetraacetic acid mobile phase at a flow
rate of 0.3 mL.min-1. Detection of peaks was done with an Agilent 1100 series
refractive index detector (Agilent Technologies, Santa Clara, CA). Quantification
was based on the external standard method (EZChrom Elite software, Version
3.3.2. SP2, Santa Clara, CA) using standards for sucrose, glucose and fructose.
All results are expressed as g.100 mL-1 of juice (BALDWIN et al., 2012a).
2.2.3 Citric acid, malic acid and ascorbic acid analyses
Organic acids were analyzed by HPLC using the same extracts that were
prepared for sugar analysis. Chromatographic separation was accomplished
with an AltechOA1000 Prevail organic acid column (9 µm, 6.5 x 300 mm)
(Grave Davison Discovery Sciences, Deerfield, IL). Samples were introduced to
the HPLC system by injecting 60 μL at a flow rate of 0.2 mL.min-1 at 35 °C and
a mobile phase of 0.005 mol.L-1 H2SO4. The analytes of interest (citric and malic
acids) were detected with a Spectra System UV 6000 LP photo diode array
detector at 215 and 245 nm (for ascorbic acid) (Thermo Fisher Scientific,
Waltham, MA). Quantification was based on the calibration curves for citric and
malic acids, expressed as g.100 mL-1 of juice (BALDWIN et al., 2017).
95
2.2.4 Secondary metabolites analyses
Concentrations of limonoids and flavonoids in orange juice were
determined by HPLC-mass spectrometry (MS) according to Baldwin et al.
(2017). Juice samples were extracted with methanol using a succession of
shaking, heating, cooling and centrifugation (BALDWIN et al., 2017). The
supernatants were combined and concentrated using a rotary evaporator model
RE111 (Buchi, Switzerland). The concentrated extract was then passed through
a 0.45 µm PTFE filter for HPLC-MS analysis. A Waters 2695 Alliance HPLC
(Waters, Medford, MA) connected in parallel with a Waters 996 Photodiode
Array (PDA) detector and a Waters/Micromass ZQ single quadrupole mass
spectrometer equipped with an electrospray ionization source was used.
Compound separations were achieved with a Waters Atlantis dC18 column (5
µm, 2.1 x 100 mm). Solvent gradient, HPLC and MS parameters were as
reported previously (BALDWIN et al., 2017). MassLynx software ver.4.1
(Micromass, Division of Waters Corp., Beverly, MA) was used for data handling.
Quantification was based on calibration curves of authentic standards of each
flavonoid and limonoid compound, expressed as g.100 mL-1 of juice.
2.3 Fractionation of phenolic compounds from orange juice
2.3.1 Preparation of phenolic compound extracts of COJ and HLBOJ
Five liters of COJ and HLBOJ were centrifuged at 27000 x g for 30 min at
5 °C. The supernatant was added to 600 g of Sepabead resin SP-207 (Supelco,
Bellefonte, PA, USA) and the mixture was shaken 1 h at 170 rpm. The liquid
was filtered and the resin was stirred with 2 L deionized water at 140 rpm for
20 min, then the water decanted. The procedure was repeated with 1 L
deionized water to remove unbound sugars. Compounds adsorbed to the resin
were removed by washing and shaking the resin three times with 2 L ethanol at
50 °C for 60 min on a shaker at 140 rpm, twice more with 1.5 L ethanol for
30 min, and finally with 1.5 L acetone/water (8:2 v/v) for 30 min. The organic
solvents used to extract the phenolic compounds were evaporated using a
rotary evaporator at 35-40 °C. The final volume was adjusted to 45 mL using
96
water/ethanol (1:1 v/v). The concentrated extract was lyophilized for 24 hours,
and the dried samples (~2 g) stored in a desiccator.
2.3.2 Fractionation of phenolic compound extracts by Fast Centrifugal Partition
Chromatography (FCPC)
Semi-preparative scale fractionation of the ‘Valencia’ juice compounds
was achieved using a fast centrifugal partition chromatography (FCPC) unit
(Kromaton, Angers, France) equipped with an A1000 rotor. The adjoining HPLC
system consisted of a Waters Delta 600 pump and controller (Waters, Milford,
MA), a sample injector (Rheodyne, Cotati, CA) with a 100 mL loop, and a
Waters 996 photodiode array detector. Fractionation was achieved using a 2 L
biphasic solvent system comprised of ethyl acetate/acetonitrile/0.5% aqueous
formic acid (1/1/2, v/v/v). The FCPC was operated in ascending mode where
stationary and mobile phases were the organic and aqueous phases,
respectively. The stationary phase was first introduced into the system with
rotors remaining stationary. Mobile phase was then pumped through the
stationary phase with the rotor spinning at 950 rpm at the flow rate of 4 mL.min–
1. Samples were prepared by dissolving the dried phenolic fraction (~ 2 g) in
equal volumes (50 mL) of the organic and aqueous phases prior to sample
injection. Fractions were then collected at 1 min intervals, and every fifth
fraction was analyzed by HPLC to help determine which fractions should be
combined. Peak elution was monitored at 330 nm. A total of five fractions, A-E,
were obtained.
2.3.3 Chemical characterization of phenolic compounds by HPLC– MS
The FCPC fractions were analyzed by the same HPLC-MS system used
for limonoids and flavonoids. Compound separations were achieved with a
Waters XBridge C8 column (5 µm, 4.6 × 150 mm). Elution conditions included
gradients of aqueous 0.5% formic acid/acetonitrile, initially 90/10 (v/v), and
changed with linear gradients to 80/20, 75/25, 60/40, 30/70, 30/70, 90/10 and
90/10 (v/v) at 10, 15, 23, 40, 45, 53, and 60 min, respectively. The same
chemical characterization was used for subsequent sub-fractions (BALDWIN et
al., 2017).
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2.3.4 Sub-fractionation of fractions A and B by HPLC
The first two FCPC fractions, A and B, were further fractionated using
semipreparative HPLC, Varian ProStar, model 210 pumps and a Prostar 335
photodiode array detector at 330 nm. Separations were achieved with an
AtlantisTM dC18 OBDTM column (5 μm, 19 x 100 mm, Waters, USA), using linear
gradients of 0.5 % v/v formic acid (solvent 1) and acetonitrile (solvent 2) as
shown in Table 1 for fractions A (Gradient 1): healthy (COJ) and HLB (HLBOJ)
and B: HLB (HLBOJ). For better separation, the gradient was slightly modified
for analysis of fraction B: healthy (COJ) (Gradient 2, Table 1). The eluted
compounds were collected in 1 min intervals and analyzed by analytical HPLC-
MS, as described above. Column fractions with similar chemical compositions
were combined. After complete solvent removal, each dried sample was stored
in a vacuum desiccator until sensory analysis.
Table 1. Mobile phases gradients (1 and 2) used to separate fractions A and B:
from healthy and huanglongbing (HLB)-affected Valencia orange juice into sub
fractions.
Time of analysis (min)
Gradient 1* Gradient 2** % Solvent 1 % Solvent 2 % Solvent 1 % Solvent 2
00:00 90 10 90 10 05:00 85 15 90 10 10:00 75 25 - - 28:00 50 50 75 25 35:00 - - 70 30 40:00 30 70 60 40 45:00 - - 30 70 48:00 30 70 - - 50:00 - - 30 70 55:00 90 10 90 10 65:00 90 10 90 10
*Gradient 1 was used to separate fraction A: healthy and HLB and fraction B: HLB into sub-
fractions; **gradient 2 was used to separate fraction B: healthy into sub-fractions. Solvent 1:
0.5% v/v formic acid; solvent 2: acetonitrile. Flow rate was set at 5 mL.min-1
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2.4 Sensory evaluation
2.4.1 Comparative sensory analysis of COJ and HLBOJ
Twelve panelists were specifically trained (12 one-hour sessions) for
orange juice descriptive analysis, with a core of seven panelists having
evaluated orange juice samples for over 5 years. Eighteen descriptors and
reference standards were developed including seven descriptors for aromatics,
five for taste, three for mouth feel and three for aftertaste (Table 2).
Only the ‘HLB flavor’ descriptor was rated according to each panelist’s
perception, based on their experience of tasting juice affected with HLB.
Descriptors were rated using a 16-point intensity scale where 0 = none, 1 = low,
7-8 = medium and 15 = high, and data were recorded using Compusense® five.
Samples were prepared as in Plotto et al. (2017) and were served in duplicate.
All taste panels took place in isolated booths equipped with computers, and
under positive air pressure and red lighting.
2.4.2 Descriptions of flavor attributes of fractions obtained from COJ and
HLBOJ
Based on HPLC-MS analyses, five FCPC fractions (A-E) were obtained
from COJ and HLBOJ. Drinking water, 4 mL, was added to each fraction and
homogenized in a vortex (Genie 2, Model No G560, Scientific Industries, USA).
The insoluble fractions were heated to 40 ± 2 °C in a hot water bath and then
completely homogenized using a vortex. This represented a stock solution,
which was tasted by two or three experienced panelists. Serial dilutions (1:1)
were performed with these fractions and subsequent sub-fractions, until the
panelists could not perceive any taste. Each team member tasted an average
volume of 0.5 mL of each dilution. Panelists cleansed palates between samples
with drinking water and consumed salted cracker as needed to dispel bitter
aftertaste. Individual observations were recorded followed by discussion of taste
impressions. The same procedure was used to taste sub-fractions from A and B
fractions. Sensory descriptors that are repeated at least two times among the
three panelists are retained.
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Table 2. Descriptors and reference standards with suggested intensity for
orange juice sensory descriptive panel, using a 16-point intensity scale*
Sensory modality
Descriptor (suggested intensity)
Reference standard
Aro
ma
tic
s (
Fla
vo
r)
Orange (7) Orange juice, 100 % Florida, Gourmet Pasteurized (Natalie’s Orchid Island Juice Company, Fort Pierce, FL).
Grapefruit (15)
Grapefruit juice, 100 % Florida, Gourmet Pasteurized (Natalie’s Orchid Island Juice Company Fort Pierce, FL).
Fruity-non-citrus (12)
A mixture of passion fruit (Welch's, Westfield, NY), mango (Frito-Lay, Inc., Dallas, TX) and pineapple (Dole Food Company Inc., Westlake Village, CA) juices and guava (Sunshine bottling Company, Doral, FL) and peach (Santiago Felippelli Conway, Miami, FL) nectars and water
Orange peel (7)
Zests from Hamlin oranges (washed and sanitized before zesting) cut in ~50 mm2 pieces (1.4 ± 0.3 g),
Green (10) A mixture of (Z)-3-hexenal (2 µg.mL-1, Sigma-Aldrich) and (Z)-3-hexenol (7 µg.mL-1, Sigma-Aldrich) in solution at 0.09 % ethanol
Stale (10) 0.005 %v/v in water of N&A Old Flavor Type, Stale (Givaudan Flavors Corp., Cincinnati, OH)
HLB flavor Any off-flavor related to HLB disease
Ta
ste
Sweet (7) 8 % sucrose (pure sugar, Publix, Lakeland, FL) in water
Sour (7) 0.2 % citric acid (≥ 99.5%, Sigma-Aldrich) in water
Umami (7) 0.08 % Monosodium glutamate (Ac’cent®, B&G Foods Inc., Parsippany, NJ)
Bitter (7) 11.5 µg.mL-1 of quinine monohydrochloride dihydrate (90 % Sigma-Aldrich) in water
Metallic (10) Canned orange juice (Ruby Kist®, 100 % Orange juice from concentrate (Clement Pappas & Co., Inc., Seabrook, NJ)
Mo
uth
fee
l
Tingly (15) Carbonated water, ClubSoda (Publix, Lakeland, FL)
Astringent (15)
Premium English Breakfast Black tea (Publix, Lakeland, FL)
Burn (7) Zests from Hamlin oranges cut in ~50 mm2 pieces (1.4 ±0.3 g), washed and sanitized before zesting.
Aft
ert
as
te Bitter (7) 11.5 µg.mL-1 of quinine monohydrochloride dihydrate (90 % Sigma-
Aldrich) in water
Astringent (15)
Premium English Breakfast black tea (Publix, Lakeland, FL)
Burning (7) Zests from Hamlin oranges cut in ~50 mm2 pieces (1.4 ±0.3 g), washed and sanitized before zesting.
*16-point intensity scale (1 = low, 7-8 = medium and 15 = high).
To determine the impacts of FCPC fractions A-E on orange juice flavor,
they were added to healthy orange juice at 120 mg.L-1, an amount estimated to
be slightly higher than normally present in orange juice, and evaluated by the
12-member trained panel. Samples were presented as pairs comprising of the
reference and a coded sample. The coded samples were the spiked samples
and included an unspiked control. Panelists rated sweetness, sourness,
bitterness, astringency and aftertaste of the coded sample on a -50 to +50 linear
100
scale in relation to the reference (negative being less, positive being more, and
“zero” as no difference from unspiked control).
2.5 Statistical analyses
All analyses were performed with two (sensory), three (limonoids and
flavonoids) or four (sugars and acids) replications. Statistical analyses were
performed as one-way ANOVA and comparison of means were undertaken by
F, Student t (P ≤ 0.01) and Tukey tests (P ≤ 0.05, 0.01 and 0.001) (Minitab®
16.2.3 Statistical Software).
3. RESULTS
The sensory evaluation of both Valencia juices, COJ and HLBOJ,
showed significant differences in all analyzed attributes (Figure 1). The positive
descriptors, “orange flavor”, “fruity-non-citrus” and “sweetness” were rated
higher for COJ compared to HLBOJ, while other descriptors representing
negative attributes such as “grapefruit flavor”, “orange peel”, “green”, “stale”,
“typical HLB flavor”, “sourness”, “bitterness”, “metallic”, “tingling”, “astringent”
and “burning”, with aftertastes of bitterness, astringency and burning, were most
frequently applied to HLBOJ samples.
The two juice types, COJ and HLBOJ were also different in that HLBOJ
had statistically higher TA and reduced pH, SSC and SSC/TA. (Figure 2).
Analysis of individual sugars revealed lower sucrose but higher glucose and
fructose levels in HLBOJ compared to COJ, with total sugars being significantly
lower. HLBOJ exhibited higher citric acid and ascorbic acid (not statistically
significant) and lower malic acid levels compared to COJ.
Levels of all secondary metabolites analyzed were higher in HLBOJ than
in COJ, except sinensetin (Figure 3), which was around 75% higher in COJ.
Nomilin, limonin, tangeretin, nobiletin and diosmin presented the greatest
difference in levels between HLBOJ and COJ corresponding to 2051, 780, 417,
231 and 229%, respectively, higher in the first.
101
Figure 1 Sensory scores (average ± standard deviation for 12 trained panelists) for Valencia orange juice from healthy (COJ) or HLB-affected (HLBOJ) fruit. Descriptors preceded with the letters “F-”, “T-”, “M-” and “A-” indicate “flavor”, “taste”, “mouthfeel” and “aftertaste”,
respectively. *, ** and *** above each pair of bars indicate significant difference between COJ and HLBOJ by ANOVA (P ≤ 0.01) and Tukey test at P ≤ 0.05, 0.01 and 0.001, respectively.
102
Figure 2. Quality attributes (average ± standard deviation for four replicates) in Valencia orange juice from healthy (COJ) or HLB-affected (HLBOJ) fruit. TA =
titratable acidity expressed in citric acid equivalent; SSC = soluble solids content. Bars followed by *, ** and *** are significantly different by ANOVA (P ≤ 0.01) and Tukey test at P ≤ 0.05, 0.01 and 0.001, respectively.
103
Figure 3. Secondary metabolites (average ± standard deviation for three replicates) in Valencia orange juice from healthy (COJ) or HLB-affected (HLBOJ) fruit. Bars followed by *, ** and *** are significantly different by ANOVA (P ≤ 0.01)
and Tukey test at P ≤ 0.05, 0.01 and 0.001, respectively. Compounds present at concentrations
lower than 10g.mL-1 are presented in the insert. HMF: heptamethoxyflavone; IKR: isosakuranetin-7-O-rutinoside or didymin; 6,8 DCGAP: 6,8-di-C-glucosyl apigenin.
Initial fractionation of the nonvolatile compounds in COJ and HLBOJ by
FCPC produced five distinct fractions (A-E). Tasting by two trained sensory
panelists revealed that the first two fractions (A and B) were the most bitter and
astringent with HLB off-flavor (data not shown). This sensory analysis was
performed by diluting with water the HLB fractions A and B to initial
concentrations of 836 mg.L-1 and 496 mg.L-1, respectively. Samples were
repeatedly tasted after successive 1:1 dilutions. Fractions A and B had
detectable residual taste after 12 and 14 dilutions, respectively, representing
final concentrations of 0.40 mg.L-1 and 0.06 mg.L-1. Fractions A-B were
subsequently added to healthy orange juice at 120 mg.L-1. The spiked orange
juice was then presented to a trained panel who evaluated taste activities of A
and B in comparison with an unspiked control juice. The panelists detected a
16% increase in bitterness for the orange juice spiked with A and a 10%
increase in astringency for the orange juice spiked with B (data not shown). The
major chemical components of A included PMFs (sinensetin, tangeretin,
heptamethoxyflavone and nobiletin), two bitter limonoid aglycones (limonin and
104
nomilin) and numerous hydroxycinnamates. Fraction B contained no PMFs but
it did contain didymin as a minor component, and additional hydroxycinnamic
acids different from those in A.
Fractions A and B were further chromatographed by preparative HPLC
to better separate and selectively detect compounds or groups of compounds
that were responsible for the bitter, astringent and harsh tastes, typical of HLB
juice. Each resulting sub-fraction was sensorially evaluated in serial dilution
tests as done previously with fractions A-E, until the taste characteristics were
imperceptible. The lowest concentration tested for each sub-fraction of A is
presented in Figure 4 and Table 3 for COJ and HLBOJ, with the lower level of
the last dilution tasted representing a stronger flavor. Results of analyses of the
sub-fractions of B are listed in Table 4 and are discussed later.
Figure 4. HPLC chromatograms of healthy (COJ) (a) or huanglongbing (HLB)-
affected (HLBOJ) (b) Valencia orange juice from fraction A showing 10 sub-
fractions with their respective lowest concentration at which taste was
perceived.
b. A-HLBOJ a. A-COJ
ppm ppm AU AU
105
Table 3. Sensory descriptors of each sub-fraction (SF) obtained from A-COJ and A-HLBOJ from healthy and huanglongbing (HLB)-
affected Valencia orange juice, respectively.
SS: stock solution; FD: final dilution; *: Sensory descriptors that are repeated at least two times among the 3 panelists are presented here; **: yerba mate is a bitter, astringent South American tea (Ilex paraguariensis St. Hilaire) that contains caffeine, phenolic compounds and saponins. HCA: hydroxycinnamate acids; SIN: sinensetin; QHME: quercetagetin hexamethyl ether; NOB: nobiletin; TMS: tetramethoxyflavone; HMF: heptamethoxyflavone; TAN: tangeretin.
SF Tentative identification of major
compounds Fraction A-COJ
Sensory descriptors*
SS FD Fraction A-HLBOJ Sensory descriptors
SS FD
(µg.mL-1) (µg.mL-1)
1 [Ferulic acid + glucaric acid] [p-Coumaric acid + glucaric acid] [Sinapinic acid + glucose] [Sinapinic acid + ferulic acid]
Caramel/honey, coffee 1275 159 Astringent, coffee, herbal, smoky 1455 182
2 [p-Coumaric acid + glucaric acid] [Ferulic acid + glucaric acid] [Sinapinic acid + ferulic acid]
Sour, acidic 3315 829 Intensely sour, intensely bitter, astringent, harsh, herbal
3390 212
3 [Ferulic acid + galactaric acid] [Sinapinic acid + ferulic acid] [Sinapinic acid + glucuronic acid] [Dimer of ferulic acid + citric acid] [Ferulic acid + sinapinic acid + glucose] [Ferulic acid + glucose]
Sour, astringent, caramel, herbal, smoky 3568 446 Intensely bitter, astringent, herbal, smoky 2370 296
4 [Ferulic acid + glucaric acid] [Sinapinic acid + glucaric acid] [Dimer of ferulic acid + glucaric acid]
Intensely astringent, sour, herbal, floral 6253 782 Intensely bitter, sour, astringent, herbal 6193 387
5 Ferulic acid [Dimer of ferulic acid + glucaric acid]
Intensely bitter, astringent, sour, herbal, burn, harsh 3493 218 Bitter, astringent, sour, herbal 2070 259
6 [Sinapinic acid + ferulic acid] Bitter, astringent, burning, metallic, herbal, floral (sweet), harsh
5266 329 Intensely bitter, astringent, burn, pungent, harsh, herbal
5075 159
7 Unknown (high mwt HCAs) [p-Coumaric acid + glucaric acid] [Ferulic acid + glucaric acid]
bitter, astringent, herbal 2099 262 Intensely bitter, sour, astringent, herbal 2548 319
8 [Sinapinic acid + ferulic acid] [Ferulic acid + glucaric acid] [Dimer of ferulic acid + glucaric acid]
Astringent, herbal, yerba mate** 1910 239 Astringent, herbal 1608 201
9 [Dimer of ferulic acid + glucaric acid] [Sinapinic acid + unknown]
Intensely bitter, astringent 4719 590 Intensely bitter, intensely harsh, pungent, herbal
3553 444
10 HCA; SIN; QHME; NOB; TMS; HMF; TAN; limonin; nomilin
Bitter, astringent, vegetable 4701 588 Intensely bitter, astringent, intense vegetable
3200 100
106
Sub-fractions from A-HLBOJ had generally stronger taste activity than
those from A-COJ as indicated by the lower concentrations at which taste was
perceived (Figure 4). Concentrations of the final dilutions (FD) tasted in sub-
fractions 2, 3, 4, 6, 9 and 10 of A-COJ were 74, 34, 51, 52, 25 and 83% higher
than the respective A-HLBOJ sub-fractions, indicating higher taste thresholds
(Table 3). Concentrations of the final dilutions (FD) tasted in A-HLBOJ sub-
fractions 1, 5, 7 and 8 were in the same range or slightly higher (13-18%) than
A-COJ sub-fractions. In fact, descriptors of sub-fractions 7 and 8 are very
similar to each other.
Overall, A-HLBOJ sub-fractions received more negative descriptors
compared to A-COJ sub-fractions. Of the five A-COJ sub-fractions classified as
bitter, two were described as intensely bitter, whereas out of the eight sub-
fractions from A-HLBOJ classified as bitter in taste, seven were described as
intensely bitter. Furthermore, in sub-fraction 3, 6, 9, and 10, initial
concentrations tasted in stock solution (SS) were slightly lower in A-HLBOJ than
in A-COJ and still presented intensely bitter descriptors. Eight sub-fractions
from A-COJ and nine sub-fractions from A-HLBOJ were described as having an
astringent mouthfeel and three sub-fractions from both samples were classified
as harsh, especially sub-fraction 9 from A-HLBOJ, which was described as
intensely harsh in spite of having lower initial concentration.
Sub-fractions 1, 3, 4 and 6 from A-COJ were characterized by positive
descriptors, such as caramel, honey and floral tastes, whereas none of the sub-
fractions from A-HLBOJ were described as such. Conversely, sub-fractions 6
and 9 from A-HLBOJ were described as pungent, whereas none of the sub-
fractions from A-COJ were. All sub-fractions from A-HLBOJ were described as
having herbal or vegetable-like tastes, with sub-fraction 10 described as having
an intense vegetable-like taste. Among sub-fractions from A-COJ, sub-fractions
1, 2 and 9 did not receive vegetable-like or herbal taste descriptors.
Sub-fractions for B-COJ and B-HLBOJ 1-10 are not quite comparable to
those of Fraction A, as the gradient had to be slightly modified to obtain better
separation of B-COJ. Nevertheless there is plenty of overlap between the B-
COJ and B-HLBOJ fractions (Table 4).
107
Table 4. Sensory descriptors and concentration of each sub-fraction obtained
from B-COJ and B-HLBOJ from healthy and huanglongbing (HLB)-affected
Valencia orange juice, respectively
Sub-fractions for Fraction B-COJ and B-HLBOJ do not exactly correspond in their retention times because a slightly different fractionation gradient was used to optimize separation in B-HLBOJ. *: The sensory descriptors are result of the final discussion between the panelists; SS: stock solution; FD: final dilution; **: yerba mate is a bitter, astringent South American tea (Ilex paraguariensis St. Hilaire) that contains caffeine, phenolic compounds and saponins.
All B-COJ and B-HLBOJ sub-fractions were described as astringent.
There were no PMFs nor limonoids in B-COJ and B-HLBOJ sub-fractions;
however, nine sub-fractions of B-HLBOJ were described as bitter, with eight
being described as intensely bitter, and six B-COJ sub-fractions as bitter, with
sub-fraction 9 described as intensely bitter. Among B-HLBOJ sub-fractions,
sub-fractions 8' and 9' had coffee taste, sub-fractions 4' and 10' had yerba mate
taste, while none of the sub-fraction from B-COJ had these descriptors. Both
sub-fractions 10' from B-COJ and B-HLBOJ received the positive descriptor
“fruity”, while only sub-fraction 1' from B-COJ received the positive descriptor
“honey”.
SF Fraction B-COJ
Sensory descriptors*
SS FD SF Fraction B-HLBOJ
Sensory descriptors
SS FD
(µg.mL-1) (µg.mL-1)
1 Honey, astringent 1413 177 1’ Sour, astringent, herbal 2150 269
2 Astringent, umami, pungent, burning
3120 390 2’ Bitter, astringent, acidic, tingly, pungent, irritating
2008 251
3 bitter, astringent, harsh, herbal
4752 594 3’ Intensely bitter, astringent, sour, tingly
5693 712
4 Sour, astringent 3070 384 4’ Intensely bitter; astringent, citric, yerba mate**
3184 816
5 bitter, astringent, pungent
2874 359 5’ Intensely bitter, astringent
2338 292
6 bitter, astringent, herbal 2752.5
344 6’ Intensely bitter, astringent, herbal
2535 634
7 bitter, sour, astringent, pungent, herbal
6981 428 7’ Intensely bitter, astringent, sour, herbal, irritating
5338 667
8 bitter, astringent 1348 337 8’ Intensely bitter, astringent, irritating, coffee
1590 398
9 Intensely bitter, astringent, harsh, herbal
6849 438 9’ Intensely bitter, astringent, irritating, coffee
5570 348
10 Citrus, fruity, astringent 3803 238 10’ Intensely bitter, astringent, yerba mate, vegetable, fruity
3183 398
108
Initial analyses of sub-fractions from A-COJ and A-HLBOJ by UV and
mass spectrometry suggest most compounds in these fractions are
hydroxycinnamates with various levels of polymerization and glycosylation
(Table 3). Only sub-fraction 10 was composed of known compounds sinensetin,
nobiletin, tangeritin, limonin and nomilin. The elution times of the majority of
hydroxycinnamates in FCPC fraction A, and hence in the sub-fractions of A-
COJ and A-HLBOJ, were typically later (15-25 min) compared to the elution
times of the hydroxycinnamates in FCPC fraction B (4-11 min) (data not
shown). This implies that the hydroxycinnamates in the A sub-fractions (Table
3) are more lipophilic than in the B sub-fractions. Consistent with this are the
frequent observations of 14 amu neutral losses from the molecular ions,
suggesting the presence of hydroxycinnamate methyl esters, generally absent
in B sub-fractions. Additionally, MS spectra of a number of the later-eluting
HCAs in FCPC A show neutral losses of ferulic and sinapinic acid subunits of
the HCAs, suggesting the occurrence of diferulic acid (neutral losses of 194
amu and 193 m/z fragment ions) and disinapinic acid (neutral mass losses of
224 amu and 223 m/z fragment ions) chemical species which are also further
conjugated to aldaric acids (evidenced by 209 and 191 m/z fragment ions)
among these compounds. Such compounds have been previously described in
sweet orange (RISCH et al., 1987; RISCH et al., 1988; HIJAZ et al., 2013;).
4. DISCUSSION
Differences between COJ and HLBOJ in both taste and compositional
analysis confirmed previous studies (BALDWIN et al., 2010; DAGULO et al.,
2010; PLOTTO et al. 2010; MASSENTI et al, 2016; KIELF et al, 2017), in which
higher levels of many secondary metabolites in juice made from oranges
symptomatic for HLB were observed. Fruit that are symptomatic of HLB tend to
be smaller, and therefore more peel components enter in the juice stream,
explaining the higher level of secondary metabolites. In general, the decrease in
sweetness in HLBOJ can be explained by lower sucrose, total sugars and
soluble solids content, together with higher citric acid. In another study,
researchers correlated the sensory descriptors sourness, umami and tingling
with some volatiles compounds, as well as tangeretin and nobiletin (PLOTTO et
109
al., 2017). Both flavones were present at higher levels in HLBOJ compared to
COJ in this study. The higher score in the sensory evaluation pertaining to
sourness can be partially explained by the higher titratable acidity and higher
citric acid content found in HLBOJ. However, sourness was also detected in
several sub-fractions of both A-COJ and A-HLBOJ extracts (Tables 3 and 4),
which suggest that some other compounds besides organic acids could be
responsible for the perception of sourness in the orange juice fractions. But
also, organic acids could have remained in the fractions and not be detected by
the HPLC system used in this study.
The increased bitterness score pertaining to HLBOJ can be partially
correlated with higher limonin, nomilin, nobiletin and tangeretin levels. The
limonin level in HLBOJ at 9.26 ± 0.87 µg.mL-1, is above its reported recognition
threshold in orange juice (4.7 µg.mL-1, DEA et al., 2013), while nomilin level at
1.08 ± 0.14 µg.mL-1, is below its reported recognition threshold (2.6 µg.mL-1,
DEA et al., 2013). In contrast, limonin and nomilin concentrations in COJ were
1.19 ± 0.03 µg.mL-1 and 0.05 ± 0.01 µg.mL-1, respectively (Figure 3), both
concentrations are below the detection thresholds (DEA et al., 2013). Higher
levels of limonin and nomilin in orange juice made with HLB symptomatic
oranges in comparison with juice made with non-symptomatic oranges have
been reported (BALDWIN et al., 2010; DAGULO et al., 2010).
HLBOJ contained higher levels of tangeretin and nobiletin than COJ,
however, the average levels were 3.06 ± 0.73 and 4.90 ± 0.08 µg.mL-1,
respectively, which were below thresholds for bitterness reported by Batenburg
et al. (2016). That particular study shows that the threshold levels of these
PMFs are above 20 µg.mL-1, and they are more abundant in citrus peel.
Hesperidin levels in HLBOJ were higher compared to COJ, which may have
contributed to the higher bitter score in the sensory evaluation as suggested by
Kiefl et al. (2017). However, in the fractionation of both samples, detectable
levels of these compounds were only in A-COJ and A-HLBOJ sub-fractions 10,
meanwhile eight other A-HLBOJ and five other A-COJ sub-fractions were
described as bitter, while lacking these compounds. In B-COJ and B-HLBOJ
sub-fractions there were no limonoids or PMFs, however eight B-HLBOJ sub-
fractions and five B-COJ sub-fractions were described as intensely bitter. This
result suggests that there are other compounds, other than limonin, nomilin,
110
tangeretin, nobiletin and hesperidin, involved with the bitter perception in
HLBOJ. These bitter-inducing compounds may likely be due to the readily
detectable hydroxycinnamates, or to other yet undetected unknowns.
5. CONCLUSION
The difference between HLBOJ and COJ was verified and partially
explained by chemical analysis, but the fractionation of HLBOJ and COJ
showed that bitterness and sourness are imparted by other compounds besides
the bitter limonoids (nomilin and limonin), bitter flavonoids (tangeretin, nobiletin
and hesperidin) and sour organic acids. The sensory descriptions of the HLBOJ
and COJ fractions implicate hydroxycinnamic acids or other compounds which
could not be identified by UV and Mass Spectrometry detectors. More studies
are warranted to determine the role of these compounds obtained from HLB-
affected orange juice, to clarify their taste activity, chemical identity and
contribution to HLB-induced off-taste.
111
CONCLUSÕES INTEGRADAS
A colheita de laranjas Valência em diferentes épocas durante uma
mesma safra influenciou nas características físico-químicas, nos teores de
compostos voláteis e metabólitos secundários do fruto. Sendo as laranjas
Valência colhidas no meio da estação as preferidas para o processamento por
apresentarem níveis ideais de SS, AT e ratio, além de reduzido conteúdo de
compostos que contribuem para o sabor amargo. Os resultados desse estudo
demonstram que a época de colheita é uma variável importante ao se estudar
os efeitos provocados pelo HLB no suco de laranja.
O suco de laranjas sintomáticas para o HLB apresenta menores teores
de açúcares totais, SS e ratio; maior acidez, elevado conteúdo de flavonoides,
limonoides e significativas diferenças sensoriais, dentre elas, os acentuados
sabores amargo e azedo. Foi demonstrado que outros compostos, além de
limonina, nomilina, tangeritina, nobiletina e hesperidina, podem contribuir para
o sabor amargo, e outros, que não os ácidos orgânicos, estão envolvidos com
o sabor azedo em suco de laranjas acometidas pelo HLB. As análises químicas
das frações de compostos não voláteis extraídos do suco de laranja, descritas
como intensamente amargas e azedas, sugerem o envolvimento de ácidos
hidroxicinâmicos ou outros compostos ainda não identificados. Além de
agrupar sistematicamente os estudos sobre os efeitos do HLB nas
características físico-químicas e sensorias de suco de laranja, o inédito
levantamento bibliográfico permitiu identificar o predomínio de pesquisas
envolvendo laranjas Valência e Hamilin em oposição às outras cultivares.
Apesar do destaque na produção das duas cultivares no Brasil e nos Estados
Unidos, o estudo das demais contribuirá para a busca de novos híbridos ou
cultivares de laranja resistentes ao HLB.
112
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PRODUÇÃO CIENTÍFICA DURANTE O DOUTORADO
Artigos completos publicados em periódicos
1. BAI,J.; BALDWIN, E.; MCCOLLUM, G.; MANTHEY, J.; PLOTTO, A.; DALA
PAULA, B.M.; GLORIA, M.B.A; WIDMER, W.; LUZIO, G.; CARMERON, R.;
NARCISO, J. Influence of harvest time on quality of ‘Valencia’ oranges and
juice, second season. Proceeding of the Florida State Horticultural Society, v.
126, p. 232-238, 2013.
Artigos a serem submetidos para publicação
1. DALA-PAULA, B.M.; PLOTTO, A.; GLÓRIA, M.B.A. Effect of Huanglongbing
(greening disease) on orange juice quality, a review.
2. DALA-PAULA, B.M.; RAITHORE, S.; MANTHEY, J.A.; BALDWIN, E.A.; BAI,
J.; ZHAO, W.; GLÓRIA, M.B.A.; PLOTTO, A. Active-taste compounds in juice
made from oranges symptomatic of Huanglongbing (HLB) greening disease.
Resumos publicados em anais de congressos
1. DALA PAULA, B.M.; RAITHORE, S; MANTHEY, J.A.; PLOTTO, A.; BAI, J.;
GLÓRIA, M.B.A.; BALDWIN, E. A deeper look into the causes of off-flavor in
orange juice affected by Huanglongbing (HLB). Journal Citrus Pathology, v. 4,
n. 1, p.8, 2017. (Apresentação de Trabalho/Conferência ou palestra).
Disponível em: <http://escholarship.org/uc/item/2cr0f2kc>.
Resumos submetidos para congressos
1. DALA PAULA, B.M.; RAITHORE, S.; MANTHEY, J.; PLOTTO, A.; BAI, J.;
GLÓRIA, M.B.A.; BALDWIN, E.A. Compounds other than limonoid aglycones
impart bitterness to orange juice affected by Huanglongbing citrus greening
disease (12th Pangborn Sensory Science Symposium –
http://www.pangbornsymposium.com/)
2. DALA PAULA, B.M.; MACHADO, G.M.; BALDWIN, E.; MANTHEY, J.A.;
PLOTTO, A.; GLÓRIA, M.B.A. Effect of Huanglonbing disease (HLB) and
different nutritional foliar treatments in amino acid and bioactive amine contents
in Hamlin orange juice (12o SLACA – A Ciência de Alimentos e seu impacto no
mundo em transformação, Campinas, UNICAMP, 2017).
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